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Patent application title:

COMPOSITIONS AND METHODS RELATED TO RECEPTOR PAIRINGS

Publication number:

US20240026014A1

Publication date:

2024-01-25

Application number:

18/019,042

Filed date:

2021-08-05

Smart Summary: New proteins have been created that can connect to specific pairs of receptors in the body. These receptors are involved in signaling processes that help cells communicate. The proteins can work with both natural receptor pairs and specially designed ones. This ability to bind to different pairs allows for more varied signaling options than what is normally possible. As a result, this innovation could lead to new ways to influence cell behavior and treat diseases. 🚀 TL;DR

Abstract:

Provided herein are receptor binding proteins that bind to either natural cytokine receptor pairs or non-natural cytokine receptor pairs to create signaling diversity beyond natural receptor pairings.

Inventors:

Patrick J. Lupardus 24 🇺🇸 Menlo Park, CA, United States
Robert Kastelein 27 🇺🇸 Menlo Park, CA, United States
Deepti Rokkam 27 🇺🇸 Menlo Park, CA, United States

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Classification:

C07K16/2866 » CPC main

Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants against receptors for cytokines, lymphokines, interferons

C07K16/2803 » CPC further

C07K2317/569 » CPC further

Immunoglobulins specific features characterized by immunoglobulin fragments variable (Fv) region, i.e. VH and/or VL Single domain, e.g. dAb, sdAb, VHH, VNAR or nanobody®

A61K2039/505 » CPC further

Medicinal preparations containing antigens or antibodies comprising antibodies

C07K16/28 IPC

Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against receptors, cell surface antigens or cell surface determinants

Description

CROSS-REFERENCE TO RELATED PATENT APPLICATIONS

This application is a national stage application under 35 U.S.C. 371 of PCT/US2021/044730, filed Aug. 5, 2021, which claims priority to U.S. Provisional Application No. 63/061,562, filed Aug. 5, 2020, U.S. Provisional Application No. 63/078,745, filed Sep. 15, 2020, and U.S. Provisional Application No. 63/135,884, filed Jan. 11, 2021, the disclosures of which are hereby incorporated by reference in their entirety for all purposes.

SEQUENCE LISTING

The instant application contains a Sequence Listing which has been submitted electronically in ASCII format and is hereby incorporated by reference in its entirety. Said ASCII copy, created on Jan. 30, 2023, is named 106249-1361943-001141US_SL.txt and is 725,670 bytes in size.

BACKGROUND OF THE DISCLOSURE

Cytokine and growth-factor ligands typically signal through homodimeric or heterodimeric cell surface receptors via Janus Kinase (JAK/TYK), or Receptor Tyrosine Kinase (RTK)-mediated transphosphorylation. However, the number of receptor dimer pairings occurring in nature is limited to those driven by natural ligands encoded within the genome.

In some instance, cytokines act as multispecific (e.g., bispecific or trispecific) ligands. Cytokines determine which receptors are included in the dimers by binding to the extracellular domain of each of the two receptors. Cytokines thus act to bridge or crosslink the receptors in a signaling complex. Cytokine receptor domain or subunit association leads to, among other effects, the activation of an intracellular JAK/STAT signaling pathway, which includes one or more of the four Janus Kinases (JAK1-3 and TYK2) (Ihle, Nature 377(6550):591-4, 1995; O'Shea and Plenge, Immunity 36(4):542-50, 2012) and several signal transducer and activator of transcription (STATs 1-6) proteins (Delgoffe, et al., Curr Opin Immunol. 23(5):632-8, 2011; Levy and Darnell, Nat Rev Mol Cell Biol. 3(9):651-62, 2002; Murray, J Immunol. 178(5):2623-9, 2007). While cytokines typically bind specifically to the extracellular domains of cell surface receptors, the JAK/TYK/STAT signaling modules are found in many combinations in endogenous cytokine receptor signaling complexes.

Given that the a ligand determines the composition of receptor domains or subunits in a receptor complex and the intracellular JAK/TYK and RTK enzymes are degenerate, the number of cytokine and growth factor receptor dimer pairings that occur in nature represents only a fraction of the total number of signaling-competent receptor pairings theoretically allowed by the system. For example, the human genome encodes for approximately forty different JAK/STAT cytokine receptors. In principle, approximately 1600 unique homodimeric and heterodimeric cytokine receptor pairs could be generated with the potential to signal through different JAK/TYK/STAT combinations (Bazan, Proc Natl Acad Sci USA. 87(18):6934-8, 1990; Huising et al., J Endocrinol. 189(1):1-25, 2006). However, as of the present knowledge, the human genome encodes for less than fifty different cytokine ligands (Bazan, Proc Natl Acad Sci USA. 87(18):6934-8, 1990; Huising et al., J Endocrinol. 189(1):1-25, 2006), limiting the scope of cytokine receptor complexes signaling to those that can be assembled by the natural ligands.

SUMMARY OF THE DISCLOSURE

In one aspect, provided herein is an IL12 receptor (IL12R) binding protein that specifically binds to IL12Rβ1 and IL12Rβ2, wherein the binding protein causes the multimerization of IL12Rβ1 and IL12Rβ2 and the multimerization results in the association of intracellular domains of IL12Rβ1 and IL12Rβ2 and intraceullar signaling, and wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL12Rβ1 (an anti-IL12Rβ1 sdAb) and a sdAb that specifically binds to IL12Rβ2 (an anti-IL12Rβ2 sdAb).

In some embodiments, the anti-IL12Rβ1 sdAb is a V_HH antibody (an anti IL12Rβ1 V_HH antibody) and/or the anti-IL12Rβ2 sdAb is a V_HH antibody (an anti IL12Rβ2 V_HH antibody). In some embodiments, the anti-IL12Rβ1 sdAb and the anti-IL12Rβ2 sdAb are joined directly or via a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids. In some embodiments, the IL12R binding protein has a reduced E_maxcompared to IL12. In some embodiments, the IL12R binding protein has an increased E_maxcompared to IL12. In some embodiments, the IL12R binding protein has a similar potency compared to that of IL12.

In another aspect, the disclosure provides a method for treating neoplastic diseases, such as cancer in a subject in need thereof, the method comprising the step of administering to the subject the IL12R binding protein as described herein, wherein the IL12R binding protein binds to and activates natural killer, CD4⁺ T cells, and/or CD8⁺ T cells. In some embodiments, the cancer is a solid tumor cancer.

In another aspect, the disclosure provides an IL27 receptor (IL27R) binding protein that specifically binds to IL27Rα subunit (IL27Rα) and glycoprotein 130 subunit (gp130), wherein the binding protein causes the multimerization of IL27Rα and gp130 and the multimerization results in the association of intracellular domains of IL27Rα and gp130 and intraceullar signaling, and wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL27Rα (an anti-IL27Rα sdAb) and a sdAb that specifically binds to gp130 (an anti-gp130 sdAb).

In some embodiments, the anti-IL27Rα sdAb is a V_HH antibody (an anti IL27Rα V_HH antibody) and/or the anti-gp130 sdAb is a V_HH antibody (an anti gp130 V_HH antibody). In some embodiments, the anti-IL27Rα sdAb and the anti-gp130 sdAb are joined directly or via a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids.

In another aspect, the disclosure provides a method for treating neoplastic diseases, such as cancer in a subject in need thereof, comprising administering to the subject the IL27R binding protein described herein, wherein the IL27R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, and/or T regulatory (Treg) cells. In some embodiments, the IL27R binding protein binds to and activates CD8⁺ T cells. In some embodiments, the IL27R binding protein binds to and activates CXCR5⁺ CD8⁺ T cells. In some embodiments, the cancer is a solid tumor cancer.

In another aspect, the disclosure provides an IL10 receptor (IL10R) binding protein that specifically binds to IL10Rα subunit (IL10Rα, also referred to herein as IL10R1) and IL10Rβ (also referred to herein as IL10R2), wherein the binding protein causes the multimerization of IL10Rα and IL10Rβ and the multimerization results in the association of intracellular domains of IL10Rα and IL10Rβ and intraceullar signaling, and wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL10Rα (an anti-IL10Rα sdAb) and a sdAb that specifically binds to IL10Rβ (an anti-IL10Rβ sdAb).

In some embodiments, the anti-IL10Rα sdAb is a V_HH antibody (an anti IL10Rα V_HH antibody) and/or the anti-IL10Rβ sdAb is a V_HH antibody (an anti IL10Rβ V_HH antibody). In some embodiments, the anti-IL10Rα sdAb and the anti-IL10Rβ sdAb are joined by a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids.

In another aspect, the disclosure provides a method for treating neoplastic diseases, such as cancer in a subject in need thereof, comprising administering to the subject the IL10R binding protein described herein, wherein the IL10R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, macrophages, and/or Treg cells. In some embodiments, the IL10R binding protein provides longer therapeutic efficacy than a pegylated IL10. In some embodiments, the cancer is a solid tumor cancer.

In other aspects, the IL10R binding proteins described herein can also be used to treat inflammatory diseases, such as Crohn's disease and ulcerative colitis, and autoimmune diseases, such as psoriasis, rheumatoid arthritis, and multiple sclerosis.

In another aspect, the disclosure provides an interferon (IFN) λ receptor (IFNλR) binding protein that specifically binds to IL10Rβ and IL28 receptor (IL28R) α subunit (IL28Rα), wherein the binding protein causes the multimerization of IL10Rβ and IL28Rα and downstream signaling, and wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL10Rβ (an anti-IL10Rβ sdAb) and a sdAb that specifically binds to IL28Rα (an anti-IL28Rα sdAb).

In some embodiments, the anti-IL10Rβ sdAb is a V_HH antibody (an anti-IL10Rβ V_HH antibody) and/or the anti-IL28Rα sdAb is a V_HH antibody (an anti IL28Rα V_HH antibody). In some embodiments, the anti-IL10Rβ sdAb and the anti-IL28Rα sdAb are joined directly or via a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids.

In another aspect, the disclosure features a method for treating an infectious disease in a subject in need thereof, comprising administering to the subject an IFNλR binding protein described herein, wherein the IFNλR binding protein binds to and activates macrophages, CD8⁺ T cells, CD4⁺ T cells, Treg cells, dendritic cells, and/or epithelial cells. In some embodiments, the IFNλR binding protein binds to and activates macrophages. In some embodiments, the infectious disease is influenza, hepatitis B, hepatitis C, or human immunodeficiency virus (HIV) infection.

In another aspect, the disclosure provides a binding protein that specifically binds to IL10Rα and IL2Rγ, wherein the binding protein causes the multimerization of IL10Rα and IL2Rγ and downstream signaling, and wherein the binding protein comprises a sdAb that specifically binds to IL10Rα (an anti-IL10Rα sdAb) and a sdAb that specifically binds to IL2Rγ (an anti-IL2Rγ sdAb).

In some embodiments, the anti-IL10Rα sdAb is a V_HH antibody (an anti-IL10Rα V_HH antibody) and/or the anti-IL2Rγ sdAb is a V_HH antibody (an anti IL2Rγ V_HH antibody). In some embodiments, the anti-IL10Rα sdAb and the anti-IL2Rγ sdAb are joined directly or via a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids.

In another aspect, the disclosure provides a method for treating neoplastic diseases, such as cancer in a subject in need thereof, comprising administering to the subject the binding protein that specifically binds to IL10Rα and IL2Rγ described herein, wherein the binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells. In some embodiments, the method does not cause anemia.

In another aspect, the disclosure provides a binding protein that specifically binds to a first receptor and a second receptor, wherein the first receptor is interferon γ receptor 1 (IFNγR1) or IL28Rα and the second receptor is preferentially expressed on myeloid cells and/or T cells, wherein the binding protein causes the multimerization of the first receptor and the second receptor and their downstream signaling, and wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to the first receptor and a sdAb that specifically binds to the second receptor.

In some embodiments, the sdAb that specifically binds to a first receptor is an anti-IFNγR1 V_HH antibody. In some embodiments, the sdAb that specifically binds to a first receptor is an anti-IL28Rα V_HH antibody. In some embodiments, the first receptor is IFNγR1 and the second receptor is IL2Rγ. In some embodiments, the first receptor is IL28Rα and the second receptor is IL2Rγ. In some embodiments, the sdAb that specifically binds to the first receptor and the sdAb that specifically binds to the second receptor are joined directly or via a peptide linker. In some embodiments, the peptide linker comprises between 1 and 50 amino acids.

In another aspect, the disclosure provides a method for treating neoplastic diseases, such as cancer in a subject in need thereof, comprising administering to the subject the binding protein that binds to a first receptor (e.g., IFNγR1 or IL28Rα) and a second receptor (e.g., a receptor preferentially expressed on myeloid cells and/or T cells) described herein, wherein the binding protein binds to and activates myeloid cells and/or T cells. In some embodiments, the binding protein binds to and activates macrophages. In some embodiments, the binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells.

DETAILED DESCRIPTION OF THE DISCLOSURE

I. Introduction

The present disclosure provides compositions useful in the pairing of cellular receptors to generate desirable effects useful in treatment of diseases. In general, binding proteins are provided that comprise at least a first domain that binds to a first receptor and a second domain that binds to a second receptor, such that upon contacting with a cell expressing the first and second receptors, the binding protein causes the functional association of the first and second receptors, thereby triggering their interaction and resulting in downstream signaling. In some embodiments, the first and second receptors occur in proximity in response to certain cytokine binding and are referred to herein as “natural” cytokine receptor pairs. In other embodiments, the binding proteins described herein bind to two receptors that do not naturally interact via binding to a naturally occurring cytokine and are referred to herein as “unnatural” cytokine receptor pairs.

Several advantages flow from the binding proteins described herein. In the case of natural cytokine receptor pairs, the natural cytokines cause the natural cytokine receptor pairs to come into proximity (i.e., by their simultaneous binding of a cytokine). However, when some of these natural cytokines are used as therapeutics in mammalian, particularly human, subjects they may also trigger a number of adverse and undesirable effects by a variety of mechanisms including the presence of the natural cytokine receptor on other cell types and the binding to those same receptor pairs on the other cell types can cause unwanted effects or trigger undesired signaling. The present disclosure is directed to manipulating the multiple effects of cytokines so that desired therapeutic signaling occurs, particularly in a desired cellular or tissue subtype, while minimizing undesired activity and/or intracellular signaling.

In some embodiment, the binding proteins described herein are designed such that the binding proteins provide the maximal desired signaling from the natural cytokine receptor pairs on the desired cell types, while the signaling from the receptors on other undesired cell types is weak such that reduced or no toxic effects result from the other undesired cell types. This can be achieved, for example, by selection of binding proteins having differing affinities or causing different E_maxfor their target receptors as compared to the affinity of a natural cytokine for the same receptors. Because different cell types respond to the binding of ligands to its cognate receptor with different sensitivity, by modulating the affinity of the ligand for the receptor compared to natural cytokine binding facilitates the stimulation of desired activities while reducing undesired activities on non-target cells. To measure downstream signaling activity, a number of methods are available. For example, in some embodiments, one can measure JAK/STAT signaling by the presence of phosphorylated receptors and/or phosphorylated STATs. In other embodiments, the expression of one or more downstream genes, whose expression levels can be affected by the level of downstream signaling caused by the binding protein, can also be measured.

In other embodiments, the binding proteins described herein provide novel signaling including, but not limited to, by bringing two receptors into proximity that generally do not interact to a significant or measurable degree under natural conditions, or signaling in specific target cell types, by binding to unnatural cytokine receptor pairs. As an example of the latter, one can obtain beneficial signaling caused by binding to the interferon γ receptor 1 (IFNγR1) or IL28Rα and a second receptor that is uniquely or preferentially expressed on myeloid or T-cells, while avoiding or reducing binding of the same receptors (e.g., IFNγR1 or IL28Rα) expressed in other cells in a human by contacting the target cells with a binding protein that comprises a first domain that specifically binds to IFNγR1 or IL28Rα and a second domain that specifically binds to a receptor uniquely or preferentially expressed on myeloid or T-cells, thereby targeting activation of IFNγR1 or IL28Rα by targeting the binding protein to these target cells (myeloid or T-cells) and limiting binding to other cells. The various receptor binding proteins described herein can be designed and tailored to bind to specific receptors, or domains or subunits thereof, that are highly expressed on the cell surface of different cell types. By binding two separate receptors, these receptor binding proteins provide a way to selectively activate or inhibit specific cell types that provide therapeutic and/or prophylactic activity useful in the treatment and/or prevention of diseases such as neoplastic diseases, such as cancer, and infectious diseases.

II. Definitions

As used herein, the term “antibody” refers collectively to: (a) glycosylated and non-glycosylated immunoglobulins (including but not limited to mammalian immunoglobulin classes IgG1, IgG2, IgG3 and IgG4) that specifically binds to target molecule and (b) immunoglobulin derivatives including but not limited to IgG(1-4)deltaC_H2, F(ab′)₂, Fab, ScFv, V_H, V_L, tetrabodies, triabodies, diabodies, dsFv, F(ab′)₃, scFv-Fc and (scFv)₂that competes with the immunoglobulin from which it was derived for binding to the target molecule. The term antibody is not restricted to immunoglobulins derived from any particular mammalian species and includes murine, human, equine, and camelids antibodies (e.g., human antibodies).

The term antibody also includes so called “single-domain antibodies” or “sdAbs,” as well as “heavy chain antibodies” or “V_HHs,” which are further defined herein. V_HHs can be obtained from immunization of camelids (including camels, llamas, and alpacas (see, e.g., Hamers-Casterman, et al. (1993) Nature 363:446-448) or by screening libraries (e.g., phage libraries) constructed in V_HH frameworks. Antibodies having a given specificity may also be derived from non-mammalian sources such as V_HHs obtained from immunization of cartilaginous fishes including, but not limited to, sharks. The term “antibody” encompasses antibodies isolatable from natural sources or from animals following immunization with an antigen and as well as engineered antibodies including monoclonal antibodies, bispecific antibodies, trispecific, chimeric antibodies, humanized antibodies, human antibodies, CDR-grafted, veneered, or deimmunized (e.g., to remove T-cell epitopes) antibodies. The term “human antibody” includes antibodies obtained from human beings as well as antibodies obtained from transgenic mammals comprising human immunoglobulin genes such that, upon stimulation with an antigen the transgenic animal produces antibodies comprising amino acid sequences characteristic of antibodies produced by human beings.

The term antibody includes both the parent antibody and its derivatives such as affinity matured, veneered, CDR grafted, humanized, camelized (in the case of V_HHs), or binding molecules comprising binding domains of antibodies (e.g., CDRs) in non-immunoglobulin scaffolds.

The term “antibody” should not be construed as limited to any particular means of synthesis and includes naturally occurring antibodies isolatable from natural sources and as well as engineered antibodies molecules that are prepared by “recombinant” means including antibodies isolated from transgenic animals that are transgenic for human immunoglobulin genes or a hybridoma prepared therefrom, antibodies isolated from a host cell transformed with a nucleic acid construct that results in expression of an antibody, antibodies isolated from a combinatorial antibody library including phage display libraries. In one embodiment, an “antibody” is a mammalian immunoglobulin. In some embodiments, the antibody is a “full length antibody” comprising variable and constant domains providing binding and effector functions.

The term antibody includes antibody conjugates comprising modifications to prolong duration of action such as fusion proteins or conjugation to polymers (e.g., PEGylated).

As used herein, the term “binding protein” refers to a protein that can bind to one or more cell surface receptors or domains or subunits thereof. In some embodiments, a binding protein specifically binds to two different receptors (or domains or subunits thereof) such that the receptors (or domains or subunits) are maintained in proximity to each other such that the receptors (or domains or subunits), including domains thereof (e.g., intracellular domains) interact with each other and result in downstream signaling.

As used herein, the term “CDR” or “complementarity determining region” is intended to mean the non-contiguous antigen combining sites found within the variable region of both heavy and light chain immunoglobulin polypeptides. CDRs have been described by Kabat et al., J. Biol. Chem. 252:6609-6616 (1977); Kabat et al., U.S. Dept. of Health and Human Services, “Sequences of proteins of immunological interest” (1991) (also referred to herein as Kabat 1991); by Chothia et al., J Mol. Biol. 196:901-917 (1987) (also referred to herein as Chothia 1987); and MacCallum et al., J. Mol. Biol. 262:732-745 (1996), where the definitions include overlapping or subsets of amino acid residues when compared against each other. Nevertheless, application of either definition to refer to a CDR of an antibody or grafted antibodies or variants thereof is intended to be within the scope of the term as defined and used herein. For purposes of the present disclosure, unless otherwise specifically identified, the positioning of CDRs2 and 3 in the variable region of an antibody follows Kabat numbering or simply, “Kabat.” The positioning of CDR1 in the variable region of an antibody follows a hybrid of Kabat and Chothia numbering schemes.

As used herein, the term “conservative amino acid substitution” refers to an amino acid replacement that changes a given amino acid to a different amino acid with similar biochemical properties (e.g., charge, hydrophobicity, and size). For example, the amino acids in each of the following groups can be considered as conservative amino acids of each other: (1) hydrophobic amino acids: alanine, isoleucine, leucine, tryptophan, phenylalanine, valine, proline, and glycine; (2) polar amino acids: glutamine, asparagine, histidine, serine, threonine, tyrosine, methionine, and cysteine; (3) basic amino acids: lysine and arginine; and (4) acidic amino acids: aspartic acid and glutamic acid.

As used herein, the term “interferon λ receptor” or “IFNλR” refers to a heterodimeric receptor formed by IL10Rβ receptor and IL28 receptor α (IL28Rα) and bound by the ligand IFNλ. Subunit IL28Rα is also referred to as IFNLR1 (IFNλ receptor 1). The human sequence of IL10Rβ is listed as UniProt ID NO. Q08334. The human sequence of IL28Rα is listed as UniProt ID NO. Q8IU57.

As used herein, the term “interferon γ receptor 1” or “IFNγR1” refers to a subunit of the heterodimeric IFNγR that is formed by subunit IFNγR1 and subunit IFNγR2 and bound by the ligand IFNγ. The amino acid sequence of the human IFNγR1 polypeptide is known and listed as UniProt ID NO. P15260.

As used herein, the term “interleukin 12 receptor” or “IL12R” refers to a heterodimeric receptor formed by subunit IL12R β1 (IL12Rβ1) and subunit IL12R β2 (IL12Rβ2) and bound by its cognate ligand IL12. The amino acid sequence of human IL12Rβ1 is known and listed as UniProt ID NO. P42701. The amino acid sequence of human IL12Rβ2 is known and listed as UniProt ID NO. Q99665.

As used herein, the term “interleukin 27 receptor” or “IL27R” refers to a heterodimeric receptor formed by subunits IL27Rα (IL27Rα) and glycoprotein 130 (gp130) and bound by the ligand IL27. The human sequence of IL27Rα is listed as UniProt ID NO. Q6UWB1. The human sequence of gp130 is listed as UniProt ID NO. Q13514.

As used herein, the term “interleukin 10 receptor” or “IL10R” refers to a tetrameric receptor formed by two IL10R α subunits (IL10Rα) and two IL10R β subunits (IL10Rβ) and bound by the ligand IL10. The amino acid sequence of human IL10Rα is listed as UniProt ID NO. Q13651. The amino acid sequence of human IL10Rβ is listed as UniProt ID NO. Q08334.

As used herein, the term “interleukin 2 receptor γ” or “IL2Rγ” refers to the γ subunit of the trimeric IL2R. IL2Rγ is also known as CD132. The amino acid sequence of human IL2Rγ is listed as UniProt ID NO. P31785.

As used herein, the term “linker” refers to a linkage between two elements, e.g., protein domains. A linker can be a covalent bond or a peptide linker. The term “bond” refers to a chemical bond, e.g., an amide bond or a disulfide bond, or any kind of bond created from a chemical reaction, e.g., chemical conjugation. The term “peptide linker” refers to an amino acid or polypeptide that may be employed to link two protein domains to provide space and/or flexibility between the two protein domains.

As used herein, the term “multimerization” refers to two or more cell surface receptors, or domains or subunits thereof, being brought in close proximity to each other such that the receptors, or domains or subunits thereof, can interact with each other and cause downstream signaling.

As used herein, the term “proximity” refers to the spatial proximity or physical distance between two cell surface receptors, or domains or subunits thereof, after a binding protein described herein binds to the two cell surface receptors, or domains or subunits thereof. In some embodiments, after the binding protein binds to the cell surface receptors, or domains or subunits thereof, the spatial proximity between the cell surface receptors, or domains or subunits thereof, can be, e.g., less than about 500 angstroms, such as e.g., a distance of about 5 angstroms to about 500 angstroms. In some embodiments, the spatial proximity amounts to less than about 5 angstroms, less than about 20 angstroms, less than about 50 angstroms, less than about 75 angstroms, less than about 100 angstroms, less than about 150 angstroms, less than about 250 angstroms, less than about 300 angstroms, less than about 350 angstroms, less than about 400 angstroms, less than about 450 angstroms, or less than about 500 angstroms. In some embodiments, the spatial proximity amounts to less than about 100 angstroms. In some embodiments, the spatial proximity amounts to less than about 50 angstroms. In some embodiments, the spatial proximity amounts to less than about 20 angstroms. In some embodiments, the spatial proximity amounts to less than about 10 angstroms. In some embodiments, the spatial proximity ranges from about 10 to 100 angstroms, from about 50 to 150 angstroms, from about 100 to 200 angstroms, from about 150 to 250 angstroms, from about 200 to 300 angstroms, from about 250 to 350 angstroms, from about 300 to 400 angstroms, from about 350 to 450 angstroms, or about 400 to 500 angstroms. In some embodiments, the spatial proximity amounts to less than about 250 angstroms, alternatively less than about 200 angstroms, alternatively less than about 150 angstroms, alternatively less than about 120 angstroms, alternatively less than about 100 angstroms, alternatively less than about 80 angstroms, alternatively less than about 70 angstroms, or alternatively less than about 50 angstroms.

As used herein, the term “downstream signaling” refers to the cellular signaling process that is caused by the interaction of two or more cell surface receptors that are brought into proximity of each other.

As used herein, the term “percent (%) sequence identity” used in the context of nucleic acids or polypeptides, refers to a sequence that has at least 50% sequence identity with a reference sequence. Alternatively, percent sequence identity can be any integer from 50% to 100%. In some embodiments, a sequence has at least 50%, 55%, 60%, 65%, 70%, 75%, 80%, 85%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, or 99% sequence identity to the reference sequence as determined with BLAST using standard parameters, as described below.

For sequence comparison, typically one sequence acts as a reference sequence, to which test sequences are compared. When using a sequence comparison algorithm, test and reference sequences are entered into a computer, subsequence coordinates are designated, if necessary, and sequence algorithm program parameters are designated. Default program parameters can be used, or alternative parameters can be designated. The sequence comparison algorithm then calculates the percent sequence identities for the test sequences relative to the reference sequence, based on the program parameters.

A comparison window includes reference to a segment of any one of the number of contiguous positions, e.g., a segment of at least 10 residues. In some embodiments, the comparison window has from 10 to 600 residues, e.g., about 10 to about 30 residues, about 10 to about 20 residues, about 50 to about 200 residues, or about 100 to about 150 residues, in which a sequence may be compared to a reference sequence of the same number of contiguous positions after the two sequences are optimally aligned.

Algorithms that are suitable for determining percent sequence identity and sequence similarity are the BLAST and BLAST 2.0 algorithms, which are described in Altschul et al. (1990) J Mol. Biol. 215: 403-410 and Altschul et al. (1977) Nucleic Acids Res. 25: 3389-3402, respectively. Software for performing BLAST analyses is publicly available through the National Center for Biotechnology Information (NCBI) web site. The algorithm involves first identifying high scoring sequence pairs (HSPs) by identifying short words of length W in the query sequence, which either match or satisfy some positive-valued threshold score T when aligned with a word of the same length in a database sequence. T is referred to as the neighborhood word score threshold (Altschul et al, supra). These initial neighborhood word hits act as seeds for initiating searches to find longer HSPs containing them. The word hits are then extended in both directions along each sequence for as far as the cumulative alignment score can be increased. Cumulative scores are calculated using, for nucleotide sequences, the parameters M (reward score for a pair of matching residues; always >0) and N (penalty score for mismatching residues; always <0). For amino acid sequences, a scoring matrix is used to calculate the cumulative score. Extension of the word hits in each direction are halted when: the cumulative alignment score falls off by the quantity X from its maximum achieved value; the cumulative score goes to zero or below, due to the accumulation of one or more negative-scoring residue alignments; or the end of either sequence is reached. The BLAST algorithm parameters W, T, and X determine the sensitivity and speed of the alignment. The BLASTN program (for nucleotide sequences) uses as defaults a word size (W) of 28, an expectation (E) of 10, M=1, N=−2, and a comparison of both strands. For amino acid sequences, the BLASTP program uses as defaults a word size (W) of 3, an expectation (E) of 10, and the BLOSUM62 scoring matrix (see Henikoff & Henikoff, Proc. Natl. Acad. Sci. USA 89:10915 (1989)).

The BLAST algorithm also performs a statistical analysis of the similarity between two sequences (see, e.g., Karlin & Altschul, Proc. Nat'l. Acad. Sci. USA 90:5873-5787 (1993)). One measure of similarity provided by the BLAST algorithm is the smallest sum probability (P(N)), which provides an indication of the probability by which a match between two nucleotide or amino acid sequences would occur by chance. For example, an amino acid sequence is considered similar to a reference sequence if the smallest sum probability in a comparison of the test amino acid sequence to the reference amino acid sequence is less than about 0.01, more preferably less than about 10⁻⁵, and most preferably less than about 10⁻²⁰.

As used herein, the term “single-domain antibody” or “sdAb” refers to an antibody having a single monomeric variable antibody domain. A sdAb is able to bind selectively to a specific antigen. A V_HH antibody, further defined below, is an example of a sdAb.

As used herein, the term “specifically bind” refers to the degree of selectivity or affinity for which one molecule binds to another. In the context of binding pairs (e.g., a binding protein described herein/receptor, a ligand/receptor, antibody/antigen, antibody/ligand, antibody/receptor binding pairs), a first molecule of a binding pair is said to specifically bind to a second molecule of a binding pair when the first molecule of the binding pair does not bind in a significant amount to other components present in the sample. A first molecule of a binding pair is said to specifically bind to a second molecule of a binding pair when the affinity of the first molecule for the second molecule is at least two-fold greater, alternatively at least five times greater, alternatively at least ten times greater, alternatively at least 20-times greater, or alternatively at least 100-times greater than the affinity of the first molecule for other components present in the sample.

In a particular embodiment, a V_HH in a bispecific V_HH²binding protein described herein binds to a receptor (e.g., the first receptor or the second receptor of the natural or non-natural receptor pairs) if the equilibrium dissociation constant between the V_HH and the receptor is greater than about 10⁶M, alternatively greater than about 10⁸M, alternatively greater than about 10¹⁰M, alternatively greater than about 10¹¹M, alternatively greater than about 10¹⁰M, greater than about 10¹²M as determined by, e.g., Scatchard analysis (Munsen, et al. 1980 Analyt. Biochem. 107:220-239). Specific binding may be assessed using techniques known in the art including but not limited to competition ELISA, BIACORE® assays and/or KINEXA® assays.

As used herein, the term “subject”, “recipient”, “individual”, or “patient”, refers to any mammalian subject for whom diagnosis, treatment, or therapy is desired, particularly humans. These terms can also be used interchangeably herein. “Mammal” for purposes of treatment refers to any animal classified as a mammal, including humans, domestic and farm animals, and zoo, sports, or pet animals, such as dogs, horses, cats, cows, sheep, goats, pigs, etc. In some embodiments, the mammal is a human being.

The terms “treat”, “treating”, treatment” and the like refer to a course of action (such as administering a binding protein described herein, or a pharmaceutical composition comprising same) initiated with respect to a subject after a disease, disorder or condition, or a symptom thereof, has been diagnosed, observed, or the like in the subject so as to eliminate, reduce, suppress, mitigate, or ameliorate, either temporarily or permanently, at least one of the underlying causes of such disease, disorder, or condition afflicting a subject, or at least one of the symptoms associated with such disease, disorder, or condition. The treatment includes a course of action taken with respect to a subject suffering from a disease where the course of action results in the inhibition (e.g., arrests the development of the disease, disorder or condition or ameliorates one or more symptoms associated therewith) of the disease in the subject.

As used herein the terms “prevent”, “preventing”, “prevention” and the like refer to a course of action initiated with respect to a subject prior to the onset of a disease, disorder, condition or symptom thereof so as to prevent, suppress, inhibit or reduce, either temporarily or permanently, a subject's risk of developing a disease, disorder, condition or the like (as determined by, for example, the absence of clinical symptoms) or delaying the onset thereof, generally in the context of a subject predisposed due to genetic, experiential or environmental factors to having a particular disease, disorder or condition. In certain instances, the terms “prevent”, “preventing”, “prevention” are also used to refer to the slowing of the progression of a disease, disorder or condition from a present its state to a more deleterious state.

As used herein, the term “V_HH” is a type of sdAb that has a single monomeric heavy chain variable antibody domain. Such antibodies can be found in or produced from Camelid mammals (e.g., camels, llamas) which are naturally devoid of light chains.

As used herein, the term “V_HH²” refers to two V_HHs that are joined together by way of a linker (e.g., a covalent bond or a peptide linker). A “bispecific V_HH²” refers to a V_HH²that has a first V_HH binding to a first receptor, or domain or subunit thereof, and a second V_HH binding to a second receptor, or domain or subunit thereof.

III. Compositions and Methods

The disclosure describes various receptor binding proteins that bind to either natural cytokine receptor pairs or domains or subunits thereof, or non-natural cytokine receptor pairs or domains or subunits thereof to create signaling diversity not observed with natural receptor pairings. The various receptor binding proteins can be screened for binding to receptor pairs or domains or subunits thereof and for signal transduction in therapeutically relevant cell types.

Receptor Binding Proteins that Bind to Natural Receptor Pairs

IL12 Receptor Binding Proteins

TheIL12 receptor (IL12R) includes subunits IL12Rβ1 and IL12Rβ2. Provided herein is an IL12R binding protein that specifically binds to IL12Rβ1 and IL12Rβ2. In some embodiments, the IL12R binding protein binds to a mammalian cell expressing both IL12Rβ1 and IL12Rβ2. In some embodiments, the IL12R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL12R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL12 or, for example, a scFv.

The IL12R binding protein can be a bispecific V_HH²that has a first V_HH binding to IL12Rβ1 (an anti-IL12Rβ1 V_HH antibody) and a second V_HH binding to IL12Rβ2 (an anti-IL12Rβ2 V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL12Rβ1 and IL12Rβ2, e.g., a natural killer or a T cell (e.g., a CD4⁺ T cells, and/or a CD8⁺ T cell).

A linker can be used to join the anti-IL12Rβ1 V_HH antibody and the anti-IL12Rβ2 V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL12Rβ1 V_HH antibody and the anti-IL12Rβ2 V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL12Rβ1 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:105-111.

The anti-IL12Rβ2 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:58-63.

The anti-IL12Rβ2 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:112-117.

In some embodiments, an IL12 receptor binding protein described herein can have an anti-IL12Rβ1 V_HH, a linker, and an anti-IL12Rβ2 V_HH as listed in Table 1 below.

TABLE 1

IL12 Receptor Binding Protein Constructs

SEQ ID NO of anti-		SEQ ID NO of anti-	Sequence of IL12 receptor
IL12Rβ1 V_HH	SEQ ID NO of	IL12Rβ2 V_HH at C-	binding protein
at N-terminus	linker	terminus	(SEQ ID NO)

105	23	112	131
105	23	113	132
105	23	114	133
105	23	115	134
105	23	116	135
105	23	117	136
106	23	112	137
106	23	113	138
106	23	114	139
106	23	115	140
106	23	116	141
106	23	117	142
107	23	112	143
107	23	113	144
107	23	114	145
107	23	115	146
107	23	116	147
107	23	117	148
108	23	112	149
108	23	113	150
108	23	114	151
108	23	115	152
108	23	116	153
108	23	117	154
109	23	112	155
109	23	113	156
109	23	114	157
109	23	115	158
109	23	116	159
109	23	117	160
112	23	105	161
112	23	106	162
112	23	107	163
112	23	108	164
112	23	109	165
113	23	105	166
113	23	106	167
113	23	107	168
113	23	108	169
113	23	109	170
114	23	105	171
114	23	106	172
114	23	107	173
114	23	108	174
114	23	109	175
115	23	105	176
115	23	106	177
115	23	107	178
115	23	108	179
115	23	109	180
116	23	105	181
116	23	106	182
116	23	107	183
116	23	108	184
116	23	109	185
117	23	105	186
117	23	106	187
117	23	107	188
117	23	108	189
117	23	109	190

In some embodiments, the IL12R binding protein has a reduced E_maxcompared to the E_maxcaused by IL12. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL12)). In some embodiments, the IL12R binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL12. In some embodiments, by varying the linker length of the IL12R binding protein, the E_maxof the IL12R binding protein can be changed. The IL12R binding protein can cause E_maxin the most desired cell types (e.g., CD8⁺ T cells), and a reduced E_maxin other cell types (e.g., natural killer cells). In some embodiments, the E_maxin natural killer cells caused by an IL12R binding protein described herein is between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 10% and 90%, between 10% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin T cells (e.g., CD8⁺ T cells) caused by the IL12R binding protein. In other embodiments, the E_maxof the IL12R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL12.

An IL12R binding protein described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), or melanoma) in a subject in need thereof. The IL12R binding protein binds to and activates natural killer, CD4⁺ T cells, and/or CD8⁺ T cells. The IL12R binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL12Rβ1 V_HH antibody and the anti-IL12Rβ2 V_HH antibody in the IL12R binding protein, the IL12R binding protein can cause a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, by varying the linker length, an IL12R binding protein can cause a higher level of downstream signaling in T cells (e.g., CD8⁺ T cells) compared to the level of downstream signaling in natural killer cells, a cell type that expresses both IL12Rβ1 and IL12Rβ2 receptors but when activated too potently can give rise to toxicities. In other embodiments, different anti-IL12Rβ1 V_HH antibodies with different binding affinities and different anti-IL12Rβ2 V_HH antibodies with different binding affinities can be combined to make different IL12R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL12Rβ1 V_HH antibody-linker-anti-IL12Rβ2 V_HH antibody, or anti-IL12Rβ2 V_HH antibody-linker-anti-IL12Rβ1 V_HH antibody). Different IL12R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, IL12R binding proteins can be partial agonists that have different activities on different cell types, e.g., T cells versus natural killer cells. For example, the selective activation of T cells over natural killer cells is desirable to avoid the toxicity associated with IL12 activated natural killer cells. In some embodiments IL12R binding protein is a partial agonist, where the partial agonist activates T cells selectively over NK cells. In some embodiments, the level of downstream signaling in T cells (e.g., CD8⁺ T cells) is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in natural killer cells.

IL27 Receptor Binding Proteins

The IL27 receptor (IL27R) includes IL27Rα subunit (IL27Rα) and glycoprotein 130 subunit (gp130). Provided herein is an IL27R binding protein that specifically binds to IL27Rα and gp130. In some embodiments, the IL27R binding protein binds to a mammalian cell expressing both IL27Rα and gp130. In some embodiments, the IL27R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL27R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL27 or, for example, a scFv.

The IL27R binding protein can be a bispecific V_HH²that has a first V_HH binding to IL27Rα (an anti-IL27Rα V_HH antibody) and a second V_HH binding to gp130 (an anti-gp130 V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL27Rα and gp130, e.g., a CD8⁺ T cells, a CD4⁺ T cells, and/or a T regulatory (Treg) cell.

A linker can be used to join the anti-IL27Rα V_HH antibody and the anti-gp130 V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL27Rα V_HH antibody and the anti-gp130 V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL27Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:70-75.

The anti-IL27Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:125-130.

The anti-gp130 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:24-29.

The anti-gp130 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:83-89.

In some embodiments, the IL27R binding protein has a reduced E_maxcompared to the E_maxcaused by IL27. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL27)). In some embodiments, the IL27R binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL27. In other embodiments, the E_maxof the IL27R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL27. In some embodiments, by varying the linker length of the IL27R binding protein, the E_maxof the IL27R binding protein can be changed. The IL27R binding protein can cause E_maxin the most desired cell types, and a reduced E_maxin other cell types.

An IL27R binding protein described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), or melanoma) and/or infectious diseases (e.g., bacterial infections and viral infections (e.g., viral infections caused by hepatitis C virus (HCV), human papillomavirus (HPV), or human immunodeficiency virus (HIV)) in a subject in need thereof. The IL27R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, and/or T regulatory (Treg) cells. The IL27R binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL27Rα V_HH antibody and the anti-gp130 V_HH antibody in the IL27R binding protein, the IL27R binding protein can cause a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, by varying the linker length, an IL27R binding protein can cause a higher level of downstream signaling in T cells (e.g., CD8+ T cells) compared to the level of downstream signaling in other cells. In other embodiments, different anti-IL27Rα V_HH antibodies with different binding affinities and different anti-gp130 V_HH antibodies with different binding affinities can be combined to make different IL27R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL27Rα V_HH antibody-linker-anti-gp130 V_HH antibody, or anti-gp130 V_HH antibody-linker-anti-IL27Rα V_HH antibody). Different IL27R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in T cells (e.g., CD8⁺ T cells) is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in other cells.

In particular, the IL27R binding protein binds to and activates CD8⁺ T cells. In some embodiments, the IL27R binding protein binds to and activates CXCR5⁺ CD8⁺ T cells. It is known that IL27 can promote and sustain a rapid division of memory-like CXCR5⁺ CD8⁺ T cells during, for example, viral infection. The CXCR5⁺ CD8⁺ T cells can sustain T cell responses during persistent infection or cancer and drive the proliferative burst of CD8⁺ T cells after anti-PD1 treatment. Accordingly, an IL27R binding protein described herein is useful to sustain and augment self-renewing T cells in chronic infections and neoplastic diseases, such as cancer.

IL10 Receptor Binding Proteins

The IL10 receptor (IL10R) includes IL10Rα subunit (IL10Rα) and IL10Rβ subunit (IL10Rβ). Provided herein is an IL10R binding protein that specifically binds to IL10Rα and IL10Rβ. In some embodiments, the IL10R binding protein binds to a mammalian cell expressing both IL10Rα and IL10Rβ. In some embodiments, the IL10R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL10R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL10 or, for example, a scFv.

The IL10R binding protein can be a bispecific V_HH²that has a first V_HH binding to IL10Rα (an anti-IL10Rα V_HH antibody) and a second V_HH binding to IL10Rβ (an anti-IL10Rβ V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL10Rα and IL10Rβ, e.g., a T cell (e.g., a CD8⁺ T cell or a CD4⁺ T cell), a macrophage, and/or a Treg cell.

A linker can be used to join the anti-IL10Rα V_HH antibody and the anti-IL10Rβ V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL10Rα V_HH antibody and the anti-IL10Rβ V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL10Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:44-50.

The anti-IL10Rα V_HH antibody can have a sequence comprising: a CDR1 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 388, 391, 394, 397, 400, 403, and 406; a CDR2 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 389, 392, 395, 398, 401, 404, and 407; and a CDR3 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 390, 393, 396, 399, 402, 405, and 408.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:51-57.

The anti-IL10Rβ V_HH antibody can have a sequence comprising: a CDR1 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 409, 412, 415, 418, 421, 424, and 427; a CDR2 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 410, 413, 416, 419, 422, 425, and 428; and a CDR3 having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity, or having 0, 1, 2, or 3 amino acid changes, optionally conservative amino acid changes relative, to the sequence of any one of SEQ ID NOS: 411, 414, 417, 420, 423, 426, and 429.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:99-104.

In some embodiments, the IL10R binding protein has a reduced E_maxcompared to the E_maxcaused by IL10. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL10)). In some embodiments, the IL10R binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL10. In some embodiments, by varying the linker length of the IL10R binding protein, the E_maxof the IL10R binding protein can be changed. The IL10R binding protein can cause E_maxin the most desired cell types (e.g., CD8⁺ T cells), and a reduced E_maxin other cell types (e.g., marcophages). In some embodiments, the E_maxin macrophages caused by an IL10R binding protein described herein is between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin T cells (e.g., CD8⁺ T cells) caused by the IL10R binding protein. In other embodiments, the E_maxof the IL10R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL10.

In some embodiments, the present disclosure provides examples of IL10 receptor binding proteins comprising anti-IL10Rα V_HH, an optional linker, and an anti-IL10Rβ2 V_HH. In some embodiments, the N-terminal V_HH of the IL-10 binding molecule is anti-IL10Rα V_HH and the C-terminal V_HH of the IL-10 receptor binding protein is anti-IL10Rβ V_HH, optionally comprising a linker between the V_HHs. In some embodiments, the N-terminal V_HH of the IL-10 receptor binding protein is an anti-IL10Rβ V_HH and the C-terminal V_HH of the IL-10 receptor binding protein is anti-IL10Rα V_HH, optionally comprising a linker between the V_HH. In some embodiments, the IL-10 receptor binding protein may provide a purification handle such as but not limited to the Ala-Ser-His-His-His-His-His-His (“ASH6”, SEQ ID NO:430) purification handle to facilitate purification of the receptor binding protein by chelating peptide immobilized metal affinity chromatography (“CP-IMAC, as described in U.S. Pat. No. 4,569,794).

As series of ninety-eight IL10 receptor binding proteins comprising anti-IL10Rα V_HH, a linker, and an anti-IL10Rβ2 V_HH and an ASH6 (SEQ ID NO: 430) purification handle (SEQ ID NOs:192-289) were prepared in substantial accordance with Examples 1-4 herein and evaluated for IL-10 activity in substantial accordance with Examples 5 and 6 herein. The arrangement of V_HH, linker and purification handle elements of these ninety-eight IL-10 receptor binding proteins is provided in Table 2 below.

TABLE 2

IL10 Receptor Binding Proteins

				C-terminal
IL10 Receptor	N-terminal		C-terminal	purification
Binding Protein	anti-IL10 V_HH	Linker	anti-IL10 V_HH	handle
(SEQ ID NO:)	(SEQ ID NO:)	(SEQ ID NO:)	(SEQ ID NO:)	(SEQ ID NO:)

192	44	23	51	430
193	44	23	52	430
194	44	23	53	430
195	44	23	54	430
196	44	23	55	430
197	44	23	56	430
198	44	23	57	430
199	45	23	51	430
200	45	23	52	430
201	45	23	53	430
202	45	23	54	430
203	45	23	55	430
204	45	23	56	430
205	45	23	57	430
206	46	23	51	430
207	46	23	52	430
208	46	23	53	430
209	46	23	54	430
210	46	23	55	430
211	46	23	56	430
212	46	23	57	430
213	47	23	51	430
214	47	23	52	430
215	47	23	53	430
216	47	23	54	430
217	47	23	55	430
218	47	23	56	430
219	47	23	57	430
220	48	23	51	430
221	48	23	52	430
222	48	24	53	430
223	48	24	54	430
224	48	24	55	430
225	48	24	56	430
226	48	24	57	430
227	49	24	51	430
228	49	24	52	430
229	49	24	53	430
230	49	24	54	430
231	49	24	55	430
232	49	24	56	430
233	49	24	57	430
234	50	24	51	430
235	50	24	52	430
236	50	24	53	430
237	50	24	54	430
238	50	24	55	430
239	50	24	56	430
240	50	24	57	430
241	51	24	44	430
242	51	24	45	430
243	51	24	46	430
244	51	24	47	430
245	51	24	48	430
246	51	24	49	430
247	51	24	50	430
248	52	24	44	430
249	52	24	45	430
250	52	24	46	430
251	52	24	47	430
252	52	24	48	430
253	52	24	49	430
254	52	24	50	430
255	53	24	44	430
256	53	24	45	430
257	53	24	46	430
258	53	24	47	430
259	53	24	48	430
260	53	24	49	430
261	53	24	50	430
262	54	24	44	430
263	54	24	45	430
264	54	24	46	430
265	54	24	47	430
266	54	24	48	430
267	54	24	49	430
268	54	24	50	430
269	55	24	44	430
270	55	24	45	430
271	55	24	46	430
272	55	24	47	430
273	55	24	48	430
274	55	24	49	430
275	55	24	50	430
276	56	24	44	430
277	56	24	45	430
278	56	24	46	430
279	56	24	47	430
280	56	24	48	430
281	56	24	49	430
282	56	24	50	430
283	57	24	44	430
284	57	24	45	430
285	57	24	46	430
286	57	24	47	430
287	57	24	48	430
288	57	24	49	430
289	57	24	50	430

As provided in more detail in the Example 3 herein, nucleic acid sequences encoding SEQ ID Nos: 192-289 were synthesized as SEQ ID Nos: 290-387 respectively and were inserted into a recombinant expression vector and expressed in HEK293 cells in 24 well place format and purified in substantial accordance with Example 4. The supernatants containing the IL-10 receptor binding proteins of SEQ ID Nos: 192-298 were evaluated for activity with unstimulated and wild-type human IL-10 as controls in substantial accordance with Examples 5 and 6 herein. The results of these experiments are provided in Table 3 below.

TABLE 3

IL10 Receptor Binding Protein Activity

TestArticle	Abs 630	Abs 630
(SEQ ID NO:)	(25 nM)	(100 nM)

Unstimulated	0.58	0.59
WildType hIL10	2.08	2.04
192	0.49	0.39
193	0.45	0.36
194	0.49	0.38
195	1.85	1.13
196	0.49	0.39
197	0.44	0.34
198	1.38	0.40
199	1.77	1.02
200	1.52	0.67
201	0.54	0.46
202	0.49	0.39
203	0.75	0.53
204	0.53	0.41
205	0.46	0.37
206	1.41	0.73
207	1.93	1.65
208	0.47	0.38
209	0.52	0.41
210	0.46	0.37
211	0.51	0.36
212	0.46	0.36
213	1.19	1.00
214	1.61	1.18
215	0.49	0.39
216	0.49	0.37
217	0.66	0.69
218	0.44	0.36
219	0.48	0.39
220	0.45	0.34
221	0.48	0.39
222	0.46	0.39
223	0.90	0.51
224	0.50	0.44
225	0.48	0.39
226	0.49	0.37
227	1.73	0.59
228	0.78	0.47
229	0.54	0.43
230	0.49	0.39
231	0.72	0.46
232	0.54	0.38
233	0.46	0.36
234	0.84	0.38
235	0.47	0.37
236	2.08	2.11
237	2.05	1.91
238	1.98	2.09
239	1.92	1.93
240	1.96	2.06
241	0.59	0.35
242	0.69	0.49
243	0.44	0.34
244	0.48	0.39
245	0.45	0.37
246	0.51	0.44
247	0.48	0.40
248	0.48	0.39
249	0.47	0.39
250	0.49	0.42
251	0.51	0.41
252	0.48	0.39
253	0.45	0.38
254	0.50	0.45
255	0.47	0.36
256	0.54	0.41
257	0.46	0.40
258	0.46	0.41
259	0.64	0.38
260	0.61	0.44
261	0.49	0.42
262	0.47	0.56
263	0.52	0.54
264	0.44	0.34
265	0.48	0.39
266	0.45	0.36
267	0.50	0.41
268	0.47	0.36
269	0.49	0.54
270	1.43	1.14
271	0.50	0.44
272	0.54	0.45
273	0.49	0.40
274	0.51	0.41
275	0.49	0.42
276	0.46	0.51
277	0.60	0.48
278	0.45	0.36
279	0.46	0.37
280	0.50	0.43
281	0.52	0.44
282	0.43	0.35
283	0.45	0.35
284	0.46	0.36
285	0.46	0.38
286	0.43	0.35
287	0.43	0.34
288	0.54	0.65
289	0.56	0.61
Unstimulated	0.58	0.59
WildType hIL10	2.08	2.04
192	0.49	0.39
193	0.45	0.36
194	0.49	0.38
195	1.85	1.13
196	0.49	0.39
197	0.44	0.34
198	1.38	0.40
199	1.77	1.02
200	1.52	0.67
201	0.54	0.46
202	0.49	0.39
203	0.75	0.53
204	0.53	0.41
205	0.46	0.37
206	1.41	0.73
207	1.93	1.65
208	0.47	0.38
209	0.52	0.41
210	0.46	0.37
211	0.51	0.36
212	0.46	0.36
213	1.19	1.00
214	1.61	1.18
215	0.49	0.39
216	0.49	0.37
217	0.66	0.69
218	0.44	0.36
219	0.48	0.39
220	0.45	0.34
221	0.48	0.39
222	0.46	0.39
223	0.90	0.51
224	0.50	0.44
225	0.48	0.39
226	0.49	0.37
227	1.73	0.59
228	0.78	0.47
229	0.54	0.43
230	0.49	0.39
231	0.72	0.46
232	0.54	0.38
233	0.46	0.36
234	0.84	0.38
235	0.47	0.37
236	2.08	2.11
237	2.05	1.91
238	1.98	2.09
239	1.92	1.93
240	1.96	2.06
241	0.59	0.35
242	0.69	0.49
243	0.44	0.34
244	0.48	0.39
245	0.45	0.37
246	0.51	0.44
247	0.48	0.40
248	0.48	0.39
249	0.47	0.39
250	0.49	0.42
251	0.51	0.41
252	0.48	0.39
253	0.45	0.38
254	0.50	0.45
255	0.47	0.36
256	0.54	0.41
257	0.46	0.40
258	0.46	0.41
259	0.64	0.38
260	0.61	0.44
261	0.49	0.42
262	0.47	0.56
263	0.52	0.54
264	0.44	0.34
265	0.48	0.39
266	0.45	0.36
267	0.50	0.41
268	0.47	0.36
269	0.49	0.54
270	1.43	1.14
271	0.50	0.44
272	0.54	0.45
273	0.49	0.40
274	0.51	0.41
275	0.49	0.42
276	0.46	0.51
277	0.60	0.48
278	0.45	0.36
279	0.46	0.37
280	0.50	0.43
281	0.52	0.44
282	0.43	0.35
283	0.45	0.35
284	0.46	0.36
285	0.46	0.38
286	0.43	0.35
287	0.43	0.34
288	0.54	0.65
289	0.56	0.61

As can be seen from the data provided above, IL-10 receptor binding proteins demonstrated significant IL-10 activity in the IL-10 activity assay (Example 4). In particular, IL-10 activity was categorized as low (above unstimulated and A₆₃₀<1), medium (A₆₃₀1-1.5) and high (A₆₃₀>1.5) based on absorbance readings. From the above data, 11 IL10R binding proteins demonstrated high activity (SEQ ID Nos: 194, 209, 210, 211, 213, 218, 226, 233, 238, 244 and 250), 4 with medium activity (SEQ ID Nos: 203, 205, 207, and 269) and 8 VHHs with low activity (SEQ ID Nos: 212, 217, 219, 224, 227, 237, 239, and 249). In some embodiments, the present disclosure provides the IL10R binding protein wherein the IL10R binding protein comprises, from amino to carboxy, a first anti-IL10R sdAb joined via a linker to a second anti-IL10R sdAb, according to the following Table 4:

	TABLE 4

	first anti-IL10R	second anti-IL10R
	sdAb SEQ ID	sdAb SEQ ID

	48	57
	49	56
	50	55
	52	46
	47	51
	51	47
	46	55
	46	56
	47	56
	46	54
	44	53
	55	44
	46	52
	45	57
	45	55
	47	55
	50	54
	48	55
	46	57
	47	57
	50	56
	49	51
	52	45
	53	44
	54	47

and wherein the IL10R binding protein further optionally comprises a linker is selected from the group consisting of SEQ ID Nos:1-23.

IL10R binding proteins described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), or melanoma) in a subject in need thereof. The IL10R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, macrophages, and/or Treg cells. In some embodiments, the IL10R binding protein described herein can provide a longer therapeutic efficacy (e.g., lower effective dose, reduced toxicity) than a wild-type or pegylated IL10. The IL10R binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL10Rα V_HH antibody and the anti-IL10Rβ V_HH antibody in the IL10R binding protein, the IL10R binding protein can cause a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments the IL10R binding protein can be a partial agonist that selectively activate T cells (e.g., CD8⁺ T cells) over macrophages. In some embodiments, activated T cells have an upregulation of IFNgamma. In some embodiments, an IL10R binding protein that is a partial agonist can suppress autoimmune inflammatory diseases such as ulcerative colitis and Crohn's disease. In some embodiments, by varying the linker length, an IL10R binding protein can cause a higher level of downstream signaling in T cells (e.g., CD8⁺ T cells) compared to the level of downstream signaling in macrophages, a cell type that expresses both IL10Rα and IL10Rβ receptors but when activated too potently can cause anemia. When the downstream signaling in macrophages is activated to a high level, these activated macrophages can then eliminate aging red blood cells, causing anemia. An IL10R binding protein can cause a higher level of downstream signaling in T cells (e.g., CD8⁺ T cells) compared to the level of downstream signaling in macrophages, such that anemia is avoided. In other embodiments, different anti-IL10Rα V_HH antibodies with different binding affinities and different anti-IL10Rβ V_HH antibodies with different binding affinities can be combined to make different IL10R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL10Rα V_HH antibody-linker-anti-IL10Rβ V_HH antibody, or anti-IL10Rβ V_HH antibody-linker-anti-IL10Rα V_HH antibody). Different IL10R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in T cells (e.g., CD8⁺ T cells) is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in macrophages.

IFNλ Receptor Binding Proteins

The interferon (IFN) λ receptor (IFNλR) includes IL10Rβ and IL28 receptor (IL28R) α subunit (IL28Rα). Provided herein is an IFNλR binding protein that specifically binds to IL10Rβ and IL28Rα. In some embodiments, the IFNλR binding protein binds to a mammalian cell expressing both IL10Rβ and IL28Rα. In some embodiments, the IFNλR binding protein can be a bispecific V_HH²as described below. In other embodiments, the IFNλR binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IFNλ or, for example, a scFv.

The IFNλR binding protein can be a bispecific V_HH²that has a first V_HH binding to IL10Rβ (an anti-IL10Rβ V_HH antibody) and a second V_HH binding to IL28Rα (an anti-IL28Rα V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL10Rβ and IL28R, e.g., a macrophage, a T cell (e.g., a CD8⁺ T cell or a CD4⁺ T cell), a Treg cell, a dendritic cell, and/or an epithelial cell.

A linker can be used to join the anti-IL10Rβ V_HH antibody and the anti-IL28Rα V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL10Rβ V_HH antibody and the anti-IL28Rα V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:51-57.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:99-104.

The anti-IL28Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:76-82.

In some embodiments, the IFNλR binding protein has a reduced E_maxcompared to the E_maxcaused by IFNλ. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IFNλ)). In some embodiments, the IFNλR binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IFNλ. In other embodiments, the E_maxof the IFNλR binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IFNλ. In some embodiments, by varying the linker length of the IFNλR binding protein, the E_maxof the IFNλR binding protein can be changed. The IFNλR binding protein can cause E_maxin the most desired cell types (e.g., macrophages), and a reduced E_maxin other cell types.

The IFNλR binding proteins of the present disclosure are useful in the treatment of an infectious disease in a subject in need thereof. The IFNλR binding protein binds to and activates macrophages, CD8⁺ T cells, CD4⁺ T cells, Treg cells, dendritic cells, and/or epithelial cells. In particular, the IFNλR binding protein binds to and activates macrophages. Examples of infectious diseases include, but are not limited to, influenza, hepatitis B, hepatitis C, and human immunodeficiency virus (HIV) infection. In some embodiments, the IFNλR binding protein can protect Kuppfer cells in the liver against the effects of an infectious disease. The IFNλR binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL10Rβ V_HH antibody and the anti-IL28Rα V_HH antibody in the IFNλR binding protein, the IFNλR binding protein can cause a higher level of downstream signaling in desired cell types (e.g., macrophages) compared to undesired cell types. In some embodiments, by varying the linker length, an IFNλR binding protein results in the modulation of downstream signaling in macrophages compared to the level of downstream signaling in other cell types. In other embodiments, different anti-IL10Rβ V_HH antibodies with different binding affinities and different anti-IL28Rα V_HH antibodies with different binding affinities can be combined to make different IFNλR binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL10Rβ V_HH antibody-linker-anti-IL28Rα V_HH antibody, or anti-IL28Rα V_HH antibody-linker-anti-IL10Rβ V_HH antibody). Different IFNλR binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in macrophages is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in other cell types.

IL23 Receptor Binding Proteins

The IL23 receptor (IL23R) includes IL12R β1 subunit (IL12Rβ1) and IL23R subunit. Provided herein is an IL23R binding protein that specifically binds to IL12Rβ1 and IL23R. In some embodiments, the IL23R binding protein binds to a mammalian cell expressing both IL12Rβ1 and IL23R. In some embodiments, the IL23R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL23R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL23 or, for example, a scFv.

The IL23R binding protein can be a bispecific V_HH²that has a first V_HH binding to IL12Rβ1 (an anti-IL12Rβ1 V_HH antibody) and a second V_HH binding to IL23R (an anti-IL23R V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL12Rβ1 and IL23R, e.g., a T cell (e.g., a CD8⁺ T cell or a CD4⁺ T cell), a macrophage, and/or a Treg cell.

A linker can be used to join the anti-IL12Rβ1 V_HH antibody and the anti-IL23R V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL12Rβ1 V_HH antibody and the anti-IL23R V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL23R V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:64-69.

The anti-IL23R V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:118-124.

In some embodiments, the IL23R binding protein has a reduced E_maxcompared to the E_maxcaused by IL23. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL23)). In some embodiments, the IL23R binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL23. In some embodiments, by varying the linker length of the IL23R binding protein, the E_maxof the IL23R binding protein can be changed. The IL23R binding protein can cause E_maxin the most desired cell types (e.g., CD8⁺ T cells), and a reduced E_maxin other cell types (e.g., marcophages). In some embodiments, the E_maxin macrophages caused by an IL23R binding protein described herein is between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin T cells (e.g., CD8⁺ T cells) caused by the IL23R binding protein. In other embodiments, the E_maxof the IL23R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL23.

An IL23R binding protein described herein are useful in wound healing. Particularly, the IL23R binding protein described herein plays an important role in initiating wound healing, e.g., healing of keratinocyte layer of the skin. The IL23R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, macrophages, and/or Treg cells. The IL23R binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL12Rβ1 V_HH antibody and the anti-IL23R V_HH antibody in the IL23R binding protein, the IL23R binding protein can cause a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments the IL23R binding protein can be a partial agonist that selectively activate T cells (e.g., CD8⁺ T cells) over macrophages. In other embodiments, different anti-IL12Rβ1 V_HH antibodies with different binding affinities and different anti-IL23R V_HH antibodies with different binding affinities can be combined to make different IL23R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL12Rβ1 V_HH antibody-linker-anti-IL23R V_HH antibody, or anti-IL23R V_HH antibody-linker-anti-IL12Rβ1 V_HH antibody). Different IL23R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in T cells (e.g., CD8⁺ T cells) is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in macrophages.

IL2 Receptor Binding Proteins

The IL2 receptor (IL2R) includes CD25 subunit (CD25; also called IL2R α subunit), CD122 subunit (CD122; also called IL2R β subunit), and CD132 subunit (CD132; also called IL2R γ subunit). Provided herein is an IL2R binding protein that specifically binds to CD122 and CD132. In some embodiments, the IL2R binding protein binds to a mammalian cell expressing both CD122 and CD132. In some embodiments, the IL2R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL2R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL2 or, for example, a scFv.

The IL2R binding protein can be a bispecific V_HH²that has a first V_HH binding to CD122 (an anti-CD122 V_HH antibody) and a second V_HH binding to CD132 (an anti-CD132 V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing CD122 and CD132, e.g., a T cell (e.g., a CD8⁺ T cell or a CD4⁺ T cell), a macrophage, and/or a Treg cell.

A linker can be used to join the anti-CD122 V_HH antibody and the anti-CD132 V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-CD122 V_HH antibody and the anti-CD132 V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-CD122 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:30-37.

The anti-CD122 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:90 and 91.

The anti-CD132 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:38-43.

The anti-CD132 V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:92-98.

In some embodiments, the IL2R binding protein has a reduced E_maxcompared to the E_maxcaused by IL2. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL2)). In some embodiments, the IL2R binding protein described herein has at least 10% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL2. In some embodiments, by varying the linker length of the IL2R binding protein, the E_maxof the IL2R binding protein can be changed. The IL2R binding protein can cause E_maxin the most desired cell types (e.g., CD8⁺ T cells), and a reduced E_maxin other cell types (e.g., marcophages). In some embodiments, the E_maxin macrophages caused by an IL2R binding protein described herein is between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin T cells (e.g., CD8⁺ T cells) caused by the IL2R binding protein. In other embodiments, the E_maxof the IL2R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL2.

An IL2R binding protein described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), melanoma, kidney cancer, or lung cancer) in a subject in need thereof. The IL2R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, macrophages, and/or Treg cells. The IL2R binding protein can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-CD122 V_HH antibody and the anti-CD132 V_HH antibody in the IL2R binding protein, the IL2R binding protein can cause a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the IL2R binding protein can be a partial agonist that selectively activate T cells (e.g., CD8⁺ T cells) over macrophages. In some embodiments, an IL2R binding protein that is a partial agonist can suppress autoimmune inflammatory diseases such as lupus, type-2 diabetes, ulcerative colitis, and Crohn's disease. In some embodiments, by varying the linker length, an IL2R binding protein can cause a higher level of downstream signaling in T cells (e.g., CD8⁺ T cells) compared to the level of downstream signaling in other cell types. In other embodiments, different anti-CD122 V_HH antibodies with different binding affinities and different anti-CD132 V_HH antibodies with different binding affinities can be combined to make different IL2R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-CD122 V_HH antibody-linker-anti-CD132 V_HH antibody, or anti-CD132 V_HH antibody-linker-anti-CD122 V_HH antibody). Different IL2R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in T cells (e.g., CD8⁺ T cells) is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in other cell types.

IL22 Receptor Binding Proteins

The IL22 receptor (IL22R) includes IL22R1 subunit (IL22R1) and IL10Rβ subunit (IL10Rβ). While IL10Rβ is expressed on a wide range of cells and especially immune cells including monocytes, T cells, B cells and NK cells, in contrast, the expression of the IL22R1 subunit of the IL22 receptor complex is primarily observed in non-immune tissues including the skin, small intestine, liver, colon, lung, kidney, and pancreas, see, e.g., Wolk, et al. (2004) Immunity 21(2):241-254. Provided herein is an IL22R binding protein that specifically binds to IL22R1 and IL10Rβ. In some embodiments, the IL22R binding protein binds to a mammalian cell expressing both IL22R1 and IL10Rβ. In some embodiments, the IL22R binding protein can be a bispecific V_HH²as described below. In other embodiments, the IL22R binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL22 or, for example, a scFv.

The IL22R binding protein can be a bispecific V_HH²that has a first V_HH binding to IL22R1 (an anti-IL22R1 V_HH antibody) and a second V_HH binding to IL10Rβ (an anti-IL10Rβ V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL22R1 and IL10Rβ, e.g., an epithelial cell. IL22R is expressed on tissue cells, and it is absent on immune cells. IL22R1 is almost exclusively expressed on cells of non-hematopoietic origin such as epithelial, renal tubular, and pancreatic ductal cells.

A linker can be used to join the anti-IL22R1 V_HH antibody and the anti-IL10Rβ V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL22R1 V_HH antibody and the anti-IL10Rβ V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:51-57.

The anti-IL10Rβ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:99-104.

In some embodiments, the IL22R binding protein has a reduced E_maxcompared to the E_maxcaused by IL22. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL22)). In some embodiments, the IL22R binding protein described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL22. In some embodiments, by varying the linker length of the IL22R binding protein, the E_maxof the IL22R binding protein can be changed.

The IL22R binding protein can cause E_maxin the most desired cell types (e.g., epithelial cells, IL22R1 expressing tumor cells, and a reduced E_maxin other cell types). In some embodiments, the E_maxin macrophages caused by an IL22R binding protein described herein is between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin epithelialis cells caused by the IL22R binding protein. In other embodiments, the E_maxof the IL22R binding protein described herein is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand, IL22.

The biological activity of IL22 is modulated by a specific endogenous antagonist, IL22 binding protein (IL22BP) which is regarded as a soluble, neutralizing decoy receptor for IL22. As wild-type IL22 possesses a higher affinity with respect to IL22BP as compared with the IL22 receptor complex, IL22BP is supposed to control IL22 biological activity in vivo. In one embodiment, the IL22R binding proteins of the present disclosure may provide preferential binding to the IL22 receptor complex versus the IL22BP avoiding the endogenous antagonism and modulation of IL22 activity derived from the presence of the endogenous IL22BP. In some embodiments, an IL22R binding protein described herein exhibits between 1% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the affinity of the natural ligand, IL22, for the IL22BP.

An IL22R binding protein described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), melanoma, kidney cancer, or lung cancer) in a subject in need thereof. The IL22R binding protein binds to and activates epithelial cells. The IL22R binding protein can trigger different levels of downstream signaling in the target cell. For example, by varying the length of the linker between the anti-IL22R1 V_HH antibody and the anti-IL10Rβ V_HH antibody in the IL22R binding protein, the IL22R binding protein can cause a differing (e.g., higher or lower) level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the IL22R binding protein can be a partial agonist that selectively activate epithelial cells. In some embodiments, an IL22R binding protein that is a partial agonist is useful in the treatment or prevention of diseases such as psoriasis, graft-versus-host disease, inflammatory diseases of the lung and airway such as lung fibrosis, ventilator induced lung injury, neoplastic disease (e.g., IL22R1-expressing tumors), liver fibrosis, diseases associated with liver injury such as alcohol toxicity (acute or chronic) steatosis, and pancreatitis, lupus, type-2 diabetes, ulcerative colitis, and Crohn's disease. In some embodiments, by varying the linker length, an IL22R binding protein can cause a higher level of downstream signaling in epithelial cells compared to the level of downstream signaling in other cell types. In other embodiments, different anti-IL22R1 V_HH antibodies with different binding affinities and different anti-IL10Rβ V_HH antibodies with different binding affinities can be combined to make different IL22R binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL22R1 V_HH antibody-linker-anti-IL10Rβ V_HH antibody, or anti-IL10Rβ V_HH antibody-linker-anti-IL22R1 V_HH antibody). Different IL22R binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in the target cell is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in other cell types or cells derived from different tissues.

Receptor Binding Proteins that Bind to Non-Natural Receptor Pairs

Receptor Binding Proteins that Bind IL10Rα and IL2Rγ

Provided herein is a binding protein that specifically binds to IL10Rα and IL2Rγ. In some embodiments, the binding protein binds to a mammalian cell expressing both IL10Rα and IL2Rγ. In some embodiments, the binding protein is a bispecific V_HH²that has a first V_HH that specifically binds to the extracellular domain of IL10Rα (an anti-IL10Rα V_HH antibody) and a second V_HH that specifically binds to the extracellular domain of IL2Rγ (an anti-IL2Rγ V_HH antibody) and causes the dimerization of the two receptor subunits and downstream signaling when bound to a cell expressing IL10Rα and IL2Rγ, e.g., a T cell (e.g., a CD8⁺ T cell and/or a CD4⁺ T cell). In some embodiments, a binding protein that specifically binds to IL10Rα and IL2Rγ can be a bispecific V_HH²as described below. In other embodiments, the binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IL10Rα or IL2Rγ or, for example, a scFv.

A linker can be used to join the anti-IL10Rα V_HH antibody and the anti-IL2Rγ V_HH antibody. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the anti-IL10Rα V_HH antibody and the anti-IL2Rγ V_HH antibody can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL10Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:44-50.

The anti-IL2Rγ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:38-43.

The anti-IL2Rγ V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:92-98.

In some embodiments, the binding protein that specifically binds to IL10Rα and IL2Rγ has a reduced E_maxcompared to the E_maxof IL10. E_maxreflects the maximum response level in a cell type that can be obtained by a ligand (e.g., a binding protein described herein or the native cytokine (e.g., IL10)). In some embodiments, the binding protein that specifically binds to IL10Rα and IL2Rγ described herein has at least 1% (e.g., between 1% and 100%, between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 10% and 90%, between 10% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxcaused by IL10. In some embodiments, by varying the linker length of the binding protein that specifically binds to IL10Rα and IL2Rγ, the E_maxof the binding protein can be changed. The binding protein can cause E_maxin the most desired cell types CD8⁺ T cells. In some embodiments, the E_maxin CD8⁺ T cells caused by a binding protein that specifically binds to IL10Rα and IL2Rγ is between 10% and 100% (e.g., between 10% and 100%, between 20% and 100%, between 30% and 100%, between 40% and 100%, between 50% and 100%, between 60% and 100%, between 70% and 100%, between 80% and 100%, between 90% and 100%, between 1% and 90%, between 1% and 80%, between 1% and 70%, between 1% and 60%, between 1% and 50%, between 1% and 40%, between 1% and 30%, between 1% and 20%, or between 1% and 10%) of the E_maxin other T cells caused by the binding protein. In other embodiments, the E_maxof the binding protein that specifically binds to IL10Rα and IL2Rγ is greater (e.g., at least 1%, 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, or 50% greater) than the E_maxof the natural ligand.

A binding protein that binds to IL10Rα and IL2Rγ as described herein is useful in the treatment of disease in a subject in need thereof including but not limited to the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), or melanoma). The binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells. In certain embodiments, the method does not cause anemia. It is known that IL10 has activities on macrophages and T cells. In some embodiments, the method provided herein uses a binding protein of the present disclosure that binds to IL10Rα and IL2Rγ resulting in the selective activation of T cells relative to activation of macrophages. The selective activation of T cells relative to macrophages is beneficial because IL10-activated macrophages can phagocytose aging red blood cells, which manifests itself as anemia in a patient receiving IL10. Binding proteins as described herein that provide for the selective substantial activation of T cells while providing a minimal activation of macrophages result in a molecule that produces lower side effects, such as anemia, relative to the native IL10 ligand. Other problems and toxicities related to IL10 activation are described in, e.g., Fioranelli and Grazia, J Integr Cardiol 1(1):2-6, 2014. Such problems can be avoided by using a binding protein of the present disclosure that specifically binds to IL10Rα and IL2Rγ.

In some embodiments, the binding protein that binds to IL10Rα and IL2Rγ can trigger different levels of downstream signaling in different cell types. For example, by varying the length of the linker between the anti-IL10Rα V_HH antibody and the anti-IL2Rγ V_HH antibody in the binding protein, the downstream signaling of the binding protein is modulated in CD8⁺ T cells compared to other T cells. In other embodiments, different anti-IL10Rα V_HH antibodies with different binding affinities and different anti-IL2Rγ V_HH antibodies with different binding affinities can be combined to make different binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., anti-IL10Rα V_HH antibody-linker-anti-IL2Rγ V_HH antibody, or anti-IL2Rγ V_HH antibody-linker-anti-IL10Rα V_HH antibody). Different binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in CD8⁺ T cells is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in other T cells.

Receptor Binding Proteins that Bind IFNγR1 or IL28Rα and Myeloid Cells and/or T Cells

Provided herein is also a binding protein that specifically binds to a first receptor and a second receptor, in which the first receptor is interferon γ receptor 1 (IFNγR1) or IL28Rα and the second receptor is preferentially expressed on myeloid cells and/or T cells. In some embodiments, the binding protein binds to a mammalian cell expressing both the first receptor and the second receptor. For example, a binding protein can selectively trigger downstream signaling in T cells if the binding protein binds to IFNγR1 as the first receptor and IL2Rγ as the second receptor expressed on T cells. In some embodiments, the binding protein can be a bispecific V_HH²as described below. In other embodiments, the binding protein can include a first domain that is a V_HH and a second domain which can be a fragment of IFNγR1 or IL28Rα or, for example, a scFv.

In one embodiment, the binding protein is a bispecific V_HH²having a first V_HH binding that specifically binds to the first receptor (e.g., an anti-IFNγR1 V_HH antibody or an anti-IL28Rα V_HH antibody) and a second V_HH that specifically binds to the second receptor and causes the dimerization of the two receptors and downstream signaling when bound to a cell expressing IFNγR1 or IL28Rα and a cell expressing the second receptor, e.g., a myeloid cell and/or T cell.

A linker can be used to join the two V_HHs. For example, a linker can simply be a covalent bond or a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A peptide linker joining the two V_HHs can be a flexible glycine-serine linker. A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

The anti-IL28Rα V_HH antibody can have a sequence having at least 90% (e.g., 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100%) sequence identity to the sequence of any one of SEQ ID NOS:76-82.

In certain embodiments of the binding protein described herein, the binding protein binds to the first receptor IFNγR1 and the second receptor IL2Rγ. In particular embodiments, the binding protein can activate T cells and avoid activating macrophages. In other embodiments, different antibodies with different binding affinities to the first receptor and different antibodies with different binding affinities to the second receptor can be combined to make different binding proteins. Further, the orientation of the two antibodies in the binding protein can also be changed to make a different binding protein (i.e., V_HH antibody to the first receptor-linker-V_HH antibody to the second receptor, or V_HH antibody to the second receptor-linker-V_HH antibody to the first receptor). Different binding proteins can be screened to find the ideal binding protein that causes a higher level of downstream signaling in desired cell types compared to undesired cell types. In some embodiments, the level of downstream signaling in T cells is at least 1.1, 1.5, 2, 3, 5, or 10 times of the level of downstream signaling in macrophages.

In certain embodiments of the binding protein described herein, the binding protein binds to the first receptor IL28Rα and the second receptor IL2Rγ.

The binding protein described herein are useful in the treatment of neoplastic diseases, such as cancer (e.g., a solid tumor cancer; e.g., non-small-cell lung carcinoma (NSCLC), renal cell carcinoma (RCC), or melanoma) in a subject in need thereof. In some embodiments, the binding protein binds to and activates myeloid cells and/or T cells. In particular embodiments, the binding protein binds to and activates macrophages. In particular embodiments, the binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells.

IV. Single-Domain Antibody and V_HH

A single-domain antibody (sdAb) is an antibody containing a single monomeric variable antibody domain. Like a full-length antibody, it is able to bind selectively to a specific antigen. The complementary determining regions (CDRs) of sdAbs are within a single-domain polypeptide. Single-domain antibodies can be engineered from heavy-chain antibodies found in camelids, which are referred to as V_HHs. Cartilaginous fishes also have heavy-chain antibodies (IgNAR, “immunoglobulin new antigen receptor”), from which single-domain antibodies referred to as V_NARScan be obtained. The dimeric variable domains from common immunoglobulin G (IgG) from humans or mice can also be split into monomers to make sdAbs. Although most research into sdAbs is currently based on heavy chain variable domains, sdAbs derived from light chains have also been shown to bind specifically to target, see, e.g., Moller et al., J Biol Chem. 285(49):38348-38361, 2010. In some embodiments, a sdAb is composed of a single monomeric light chain variable antibody domain.

A sdAb can be a heavy chain antibody (V_HH). A V_HH is a type of sdAb that has a single monomeric heavy chain variable antibody domain. Similar to a traditional antibody, a V_HH is able to bind selectively to a specific antigen. A binding protein described herein can include two V_HHs (e.g., V_HH²) joined together by a linker (e.g., a peptide linker). The binding protein can be a bispecific V_HH²that includes a first V_HH binding to a first receptor or domain or subunit thereof and a second V_HH binding to a second receptor or domain or subunit thereof, in which the two V_HHs are joined by a linker.

An exemplary V_HH has a molecular weight of approximately 12-15 kDa which is much smaller than traditional mammalian antibodies (150-160 kDa) composed of two heavy chains and two light chains. V_HHs can be found in or produced from Camelidae mammals (e.g., camels, llamas, dromedary, alpaca, and guanaco) which are naturally devoid of light chains. Descriptions of sdAbs and V_HHS can be found in, e.g., De Greve et al., Curr Opin Biotechnol. 61:96-101, 2019; Ciccarese, et al., Front Genet. 10:997, 2019; Chanier and Chames, Antibodies (Basel) 8(1), 2019; and De Vlieger et al., Antibodies (Basel) 8(1), 2018.

To prepare a binding protein that is a bispecific V_HH², in some embodiments, the two V_HHs can be synthesized separately, then joined together by a linker. Alternatively, the bispecific V_HH²can be synthesized as a fusion protein. V_HHs having different binding activities and receptor targets can be paired to make a bispecific V_HH². The binding proteins can be screened for signal transduction on cells carrying one or both relevant receptors.

V. Linkers

As previously described, the binding domains of the binding proteins of the present disclosure may be joined contiguously (e.g., the C-terminal amino acid of the first V_HH in the binding protein to the N-terminal amino acid of the second V_HH in the binding protein) or the binding domains of the binding protein may optionally be joined via a linker. A linker is a linkage between two elements, e.g., protein domains. In a bispecific V_HH²binding protein described herein, a linker is a linkage between the two V_HHs in the binding protein. A linker can be a covalent bond or a peptide linker. In some embodiments, the two V_HHs in a binding protein are joined directly (i.e., via a covalent bond). The length of the linker between two V_HHs in a binding protein can be used to modulate the proximity of the two V_HHs of the binding protein. By varying the length of the linker, the overall size and length of the binding protein can be tailored to bind to specific cell receptors or domains or subunits thereof. For example, if the binding protein is designed to bind to two receptors or domains or subunits thereof that are located close to each other on the same cell, then a short linker can be used. In another example, if the binding protein is designed to bind to two receptors or domains or subunits there of that are located on two different cells, then a long linker can be used.

In some embodiments, the linker is a peptide linker. A peptide linker can include between 1 and 50 amino acids (e.g., between 2 and 50, between 5 and 50, between 10 and 50, between 15 and 50, between 20 and 50, between 25 and 50, between 30 and 50, between 35 and 50, between 40 and 50, between 45 and 50, between 2 and 45, between 2 and 40, between 2 and 35, between 2 and 30, between 2 and 25, between 2 and 20, between 2 and 15, between 2 and 10, between 2 and 5 amino acids). A linker can also be a chemical linker, such as a synthetic polymer, e.g., a polyethylene glycol (PEG) polymer.

In some embodiments, a linker joins the C-terminus of the first V_HH in the binding protein to the N-terminus of the second V_HH in the binding protein. In other embodiments, a linker joins the C-terminus of the second V_HH in the binding protein to the N-terminus of the first V_HH in the binding protein.

Suitable peptide linkers are known in the art, and include, for example, peptide linkers containing flexible amino acid residues such as glycine and serine. In certain embodiments, a peptide linker can contain motifs, e.g., multiple or repeating motifs, of GS, GGS, GGGGS (SEQ ID NO: 1), GGGGGS (SEQ ID NO:2), GGSG (SEQ ID NO:3), or SGGG (SEQ ID NO:4). In certain embodiments, a peptide linker can contain 2 to 12 amino acids including motifs of GS, e.g., GS, GSGS (SEQ ID NO:5), GSGSGS (SEQ ID NO:6), GSGSGSGS (SEQ ID NO:191), GSGSGSGSGS (SEQ ID NO:7), or GSGSGSGSGSGS (SEQ ID NO:8). In certain other embodiments, a peptide linker can contain 3 to 12 amino acids including motifs of GGS, e.g., GGS, GGSGGS (SEQ ID NO:9), GGSGGSGGS (SEQ ID NO:10), and GGSGGSGGSGGS (SEQ ID NO:11). In yet other embodiments, a peptide linker can contain 4 to 20 amino acids including motifs of GGSG (SEQ ID NO:3), e.g., GGSGGGSG (SEQ ID NO:12), GGSGGGSGGGSG (SEQ ID NO:13), GGSGGGSGGGSGGGSG (SEQ ID NO:14), or GGSGGGSGGGSGGGSGGGSG (SEQ ID NO: 15). In other embodiments, a peptide linker can contain motifs of GGGGS (SEQ ID NO: 1), e.g., GGGGSGGGGS (SEQ ID NO:16) or GGGGSGGGGSGGGGS (SEQ ID NO:17).

VI. Modifications to Extend Duration of Action In Vivo

The binding proteins described herein can be modified to provide for an extended lifetime in vivo and/or extended duration of action in a subject. In some embodiments, the binding protein can be conjugated to carrier molecules to provide desired pharmacological properties such as an extended half-life. In some embodiments, the binding protein can be covalently linked to the Fc domain of IgG, albumin, or other molecules to extend its half-life, e.g., by pegylation, glycosylation, and the like as known in the art.

In some embodiments, the binding protein is conjugated to a functional domain of an Fc-fusion chimeric polypeptide molecule. Fc fusion conjugates have been shown to increase the systemic half-life of biopharmaceuticals, and thus the biopharmaceutical product can require less frequent administration. Fc binds to the neonatal Fc receptor (FcRn) in endothelial cells that line the blood vessels, and, upon binding, the Fc fusion molecule is protected from degradation and re-released into the circulation, keeping the molecule in circulation longer. This Fc binding is believed to be the mechanism by which endogenous IgG retains its long plasma half-life. More recent Fc-fusion technology links a single copy of a biopharmaceutical to the Fc region of an antibody to optimize the pharmacokinetic and pharmacodynamic properties of the biopharmaceutical as compared to traditional Fc-fusion conjugates. The “Fc region” useful in the preparation of Fc fusions can be a naturally occurring or synthetic polypeptide that is homologous to an IgG C-terminal domain produced by digestion of IgG with papain. IgG Fc has a molecular weight of approximately 50 kDa. The binding protein described herein can be conjugated to the entire Fc region, or a smaller portion that retains the ability to extend the circulating half-life of a chimeric polypeptide of which it is a part. In addition, full-length or fragmented Fc regions can be variants of the wild-type molecule. In a typical presentation, each monomer of the dimeric Fc can carry a heterologous polypeptide, the heterologous polypeptides being the same or different.

In some embodiments, when the binding protein described herein is to be administered in the format of an Fc fusion, particularly in those situations when the polypeptide chains conjugated to each subunit of the Fc dimer are different, the Fc fusion may be engineered to possess a “knob-into-hole modification.” The knob-into-hole modification is more fully described in Ridgway, et al. (1996) Protein Engineering 9(7):617-621 and U.S. Pat. No. 5,731,168, issued Mar. 24, 1998. The knob-into-hole modification refers to a modification at the interface between two immunoglobulin heavy chains in the CH3 domain, wherein: i) in a CH3 domain of a first heavy chain, an amino acid residue is replaced with an amino acid residue having a larger side chain (e.g., tyrosine or tryptophan) creating a projection from the surface (“knob”), and ii) in the CH3 domain of a second heavy chain, an amino acid residue is replaced with an amino acid residue having a smaller side chain (e.g., alanine or threonine), thereby generating a cavity (“hole”) at interface in the second CH3 domain within which the protruding side chain of the first CH3 domain (“knob”) is received by the cavity in the second CH3 domain. In one embodiment, the “knob-into-hole modification” comprises the amino acid substitution T366W and optionally the amino acid substitution S354C in one of the antibody heavy chains, and the amino acid substitutions T366S, L368A, Y407V and optionally Y349C in the other one of the antibody heavy chains. Furthermore, the Fc domains may be modified by the introduction of cysteine residues at positions 5354 and Y349 which results in a stabilizing disulfide bridge between the two antibody heavy chains in the Fc region (Carter, et al. (2001) Immunol Methods 248, 7-15). The knob-into-hole format is used to facilitate the expression of a first polypeptide on a first Fc monomer with a “knob” modification and a second polypeptide on the second Fc monomer possessing a “hole” modification to facilitate the expression of heterodimeric polypeptide conjugates.

In some embodiments, the binding protein can be conjugated to one or more water-soluble polymers. Examples of water soluble polymers useful in the practice of the present disclosure include polyethylene glycol (PEG), poly-propylene glycol (PPG), polysaccharides (polyvinylpyrrolidone, copolymers of ethylene glycol and propylene glycol, poly(oxyethylated polyol), polyolefinic alcohol), polysaccharides), poly-alpha-hydroxy acid), polyvinyl alcohol (PVA), polyphosphazene, polyoxazolines (POZ), poly(N-acryloylmorpholine), or a combination thereof.

In some embodiments, binding protein can be conjugated to one or more polyethylene glycol molecules or “PEGylated.” Although the method or site of PEG attachment to the binding protein may vary, in certain embodiments the PEGylation does not alter, or only minimally alters, the activity of the binding protein.

In some embodiments, selective PEGylation of the binding protein, for example, by the incorporation of non-natural amino acids having side chains to facilitate selective PEG conjugation, may be employed. Specific PEGylation sites can be chosen such that PEGylation of the binding protein does not affect its binding to the target receptors.

In certain embodiments, the increase in half-life is greater than any decrease in biological activity. PEGs suitable for conjugation to a polypeptide sequence are generally soluble in water at room temperature, and have the general formula R(O—CH₂—CH₂)_nO—R, where R is hydrogen or a protective group such as an alkyl or an alkanol group, and where n is an integer from 1 to 1000. When R is a protective group, it generally has from 1 to 8 carbons. The PEG conjugated to the polypeptide sequence can be linear or branched. Branched PEG derivatives, “star-PEGs” and multi-armed PEGs are contemplated by the present disclosure.

A molecular weight of the PEG used in the present disclosure is not restricted to any particular range. The PEG component of the binding protein can have a molecular mass greater than about 5 kDa, greater than about 10 kDa, greater than about 15 kDa, greater than about 20 kDa, greater than about 30 kDa, greater than about 40 kDa, or greater than about 50 kDa. In some embodiments, the molecular mass is from about 5 kDa to about 10 kDa, from about 5 kDa to about 15 kDa, from about 5 kDa to about 20 kDa, from about 10 kDa to about 15 kDa, from about 10 kDa to about 20 kDa, from about 10 kDa to about 25 kDa, or from about 10 kDa to about 30 kDa. Linear or branched PEG molecules having molecular weights from about 2,000 to about 80,000 daltons, alternatively about 2,000 to about 70,000 daltons, alternatively about 5,000 to about 50,000 daltons, alternatively about 10,000 to about 50,000 daltons, alternatively about 20,000 to about 50,000 daltons, alternatively about 30,000 to about 50,000 daltons, alternatively about 20,000 to about 40,000 daltons, or alternatively about 30,000 to about 40,000 daltons. In one embodiment of the disclosure, the PEG is a 40 kD branched PEG comprising two 20 kD arms.

The present disclosure also contemplates compositions of conjugates wherein the PEGs have different n values, and thus the various different PEGs are present in specific ratios. For example, some compositions comprise a mixture of conjugates where n=1, 2, 3 and 4. In some compositions, the percentage of conjugates where n=1 is 18-25%, the percentage of conjugates where n=2 is 50-66%, the percentage of conjugates where n=3 is 12-16%, and the percentage of conjugates where n=4 is up to 5%. Such compositions can be produced by reaction conditions and purification methods known in the art. Chromatography may be used to resolve conjugate fractions, and a fraction is then identified which contains the conjugate having, for example, the desired number of PEGs attached, purified free from unmodified protein sequences and from conjugates having other numbers of PEGs attached.

PEGs suitable for conjugation to a polypeptide sequence are generally soluble in water at room temperature, and have the general formula R(O—CH₂—CH₂)_nO—R, where R is hydrogen or a protective group such as an alkyl or an alkanol group, and where n is an integer from 1 to 1000. When R is a protective group, it generally has from 1 to 8 carbons.

Two widely used first generation activated monomethoxy PEGs (mPEGs) are succinimdyl carbonate PEG (SC-PEG; see, e.g., Zalipsky, et al. (1992) Biotehnol. Appl. Biochem 15:100-114) and benzotriazole carbonate PEG (BTC-PEG; see, e.g., Dolence, et al. U.S. Pat. No. 5,650,234), which react preferentially with lysine residues to form a carbamate linkage but are also known to react with histidine and tyrosine residues. Use of a PEG-aldehyde linker targets a single site on the N-terminus of a polypeptide through reductive amination.

Pegylation most frequently occurs at the α-amino group at the N-terminus of the polypeptide, the epsilon amino group on the side chain of lysine residues, and the imidazole group on the side chain of histidine residues. Since most recombinant polypeptides possess a single alpha and a number of epsilon amino and imidazole groups, numerous positional isomers can be generated depending on the linker chemistry. General PEGylation strategies known in the art can be applied herein.

The PEG can be bound to a binding protein of the present disclosure via a terminal reactive group (a “spacer”) which mediates a bond between the free amino or carboxyl groups of one or more of the polypeptide sequences and polyethylene glycol. The PEG having the spacer which can be bound to the free amino group includes N-hydroxysuccinylimide polyethylene glycol, which can be prepared by activating succinic acid ester of polyethylene glycol with N-hydroxysuccinylimide.

In some embodiments, the PEGylation of the binding proteins is facilitated by the incorporation of non-natural amino acids bearing unique side chains to facilitate site specific PEGylation. The incorporation of non-natural amino acids into polypeptides to provide functional moieties to achieve site specific PEGylation of such polypeptides is known in the art. See e.g., Ptacin et al., PCT International Application No. PCT/US2018/045257 filed Aug. 3, 2018 and published Feb. 7, 2019 as International Publication Number WO 2019/028419A1.

The PEG conjugated to the polypeptide sequence can be linear or branched. Branched PEG derivatives, “star-PEGs” and multi-armed PEGs are contemplated by the present disclosure. Specific embodiments PEGs useful in the practice of the present disclosure include a 10 kDa linear PEG-aldehyde (e.g., Sunbright® ME-100AL, NOF America Corporation, One North Broadway, White Plains, NY 10601 USA), 10 kDa linear PEG-NHS ester (e.g., Sunbright® ME-100CS, Sunbright® ME-100AS, Sunbright® ME-100GS, Sunbright® ME-100HS, NOF), a 20 kDa linear PEG-aldehyde (e.g., Sunbright® ME-200AL, NOF), a 20 kDa linear PEG-NHS ester (e.g., Sunbright® ME-200CS, Sunbright® ME-200AS, Sunbright® ME-200GS, Sunbright® ME-200HS, NOF), a 20 kDa 2-arm branched PEG-aldehyde the 20 kDA PEG-aldehyde comprising two 10 kDA linear PEG molecules (e.g., Sunbright® GL2-200AL3, NOF), a 20 kDa 2-arm branched PEG-NHS ester the 20 kDA PEG-NHS ester comprising two 10 kDA linear PEG molecules (e.g., Sunbright® GL2-200TS, Sunbright® GL200GS2, NOF), a 40 kDa 2-arm branched PEG-aldehyde the 40 kDA PEG-aldehyde comprising two 20 kDA linear PEG molecules (e.g., Sunbright® GL2-400AL3), a 40 kDa 2-arm branched PEG-NHS ester the 40 kDA PEG-NHS ester comprising two 20 kDA linear PEG molecules (e.g., Sunbright® GL2-400AL3, Sunbright® GL2-400GS2, NOF), a linear 30 kDa PEG-aldehyde (e.g., Sunbright® ME-300AL) and a linear 30 kDa PEG-NHS ester.

In some embodiments, a linker can used to join the binding protein and the PEG molecule. Suitable linkers include “flexible linkers” which are generally of sufficient length to permit some movement between the modified polypeptide sequences and the linked components and molecules. The linker molecules are generally about 6-50 atoms long. The linker molecules may also be, for example, aryl acetylene, ethylene glycol oligomers containing 2-10 monomer units, diamines, diacids, amino acids, or combinations thereof. Suitable linkers can be readily selected and can be of any suitable length, such as 1 amino acid (e.g., Gly), 2, 3, 4, 5, 6, 7, 8, 9, 10, 10-20, 20-30, 30-50 or more than 50 amino acids.

Examples of flexible linkers include glycine polymers (G)n, glycine-alanine polymers, alanine-serine polymers, glycine-serine polymers (for example, (GmSo)n (SEQ ID NO: 431), (GSGGS)n (SEQ ID NO: 432), (GmSoGm)n (SEQ ID NO: 433), (GmSoGmSoGm)n (SEQ ID NO: 434), (GSGGSm)n (SEQ ID NO: 435), (GSGSmG)n (SEQ ID NO: 436) and (GGGSm)n (SEQ ID NO: 437), and combinations thereof, where m, n, and o are each independently selected from an integer of at least 1 to 20, e.g., 1-18, 216, 3-14, 4-12, 5-10, 1, 2, 3, 4, 5, 6, 7, 8, 9, or 10), and other flexible linkers. Glycine and glycine-serine polymers are relatively unstructured, and therefore may serve as a neutral tether between components. Examples of flexible linkers include, but are not limited to GGSG (SEQ ID NO:3), GGSGG (SEQ ID NO:18), GSGSG (SEQ ID NO:19), GSGGG (SEQ ID NO:20), GGGSG (SEQ ID NO:21), and GSSSG (SEQ ID NO:22). Other examples of flexible linkers are described in Section V.

Additional examples of flexible linkers include glycine polymers (G)n or glycine-serine polymers (e.g., (GS)n (SEQ ID NO: 438), (GSGGS)n (SEQ ID NO: 439), (GGGS)n (SEQ ID NO: 440) and (GGGGS)n (SEQ ID NO: 441), where n=1 to 50, for example, 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 10-20, 20-30, 30-50). Exemplary flexible linkers include, but are not limited to GGGS (SEQ ID NO:23), GGGGS (SEQ ID NO:1), GGSG (SEQ ID NO:3), GGSGG (SEQ ID NO:18), GSGSG (SEQ ID NO:19), GSGGG (SEQ ID NO:20), GGGSG (SEQ ID NO:21), and GSSSG (SEQ ID NO:22). A multimer (e.g., 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 10-20, 20-30, or 30-50) of these linker sequences may be linked together to provide flexible linkers that may be used to conjugate two molecules. Alternative to a polypeptide linker, the linker can be a chemical linker, e.g., a PEG-aldehyde linker. In some embodiments, the binding protein is acetylated at the N-terminus by enzymatic reaction with N-terminal acetyltransferase and, for example, acetyl CoA. Alternatively, or in addition to N-terminal acetylation, the binding protein can be acetylated at one or more lysine residues, e.g., by enzymatic reaction with a lysine acetyltransferase. See, for example Choudhary et al. (2009) Science 325 (5942):834-840.

In other embodiments, the binding protein can be modified to include an additional polypeptide sequence that functions as an antigenic tag, such as a FLAG sequence. FLAG sequences are recognized by biotinylated, highly specific, anti-FLAG antibodies, as described herein (see e.g., Blanar et al. (1992) Science 256:1014 and LeClair, et al. (1992) PNAS-USA 89:8145). In some embodiments, the binding protein further comprises a C-terminal c-myc epitope tag.

In some embodiments, the binding protein is expressed as a fusion protein with an albumin molecule (e.g., human serum albumin) which is known in the art to facilitate extended exposure in vivo.

In some embodiment, the binding proteins (including fusion proteins of the binding proteins) of the present disclosure are expressed as a fusion protein with one or more transition metal chelating polypeptide sequences. The incorporation of such a transition metal chelating domain facilitates purification immobilized metal affinity chromatography (IMAC) as described in Smith, et al. U.S. Pat. No. 4,569,794 issued Feb. 11, 1986. Examples of transition metal chelating polypeptides useful in the practice of the present disclosure are described in Smith, et al. supra and Dobeli, et al. U.S. Pat. No. 5,320,663 issued May 10, 1995, the entire teachings of which are hereby incorporated by reference. Particular transition metal chelating polypeptides useful in the practice of the present disclosure are peptides comprising 3-6 contiguous histidine residues (SEQ ID NO: 443) such as a six-histidine peptide (His)₆(SEQ ID NO: 442) and are frequently referred to in the art as “His-tags.”

The foregoing fusion proteins may be readily produced by recombinant DNA methodology by techniques known in the art by constructing a recombinant vector comprising a nucleic acid sequence comprising a nucleic acid sequence encoding the binding protein in frame with a nucleic acid sequence encoding the fusion partner either at the N-terminus or C-terminus of the binding protein, the sequence optionally further comprising a nucleic acid sequence in frame encoding a linker or spacer polypeptide.

VII. Pharmaceutical Composition

The binding proteins of the present disclosure may be administered to a subject in a pharmaceutically acceptable dosage form. The preferred formulation depends on the intended mode of administration and therapeutic application. Pharmaceutical dosage forms of the binding proteins described herein comprise physiologically acceptable carriers that are inherently non-toxic and non-therapeutic. Examples of such carriers include ion exchangers, alumina, aluminum stearate, lecithin, serum proteins, such as human serum albumin, buffer substances such as phosphates, glycine, sorbic acid, potassium sorbate, partial glyceride mixtures of saturated vegetable fatty acids, water, salts, or electrolytes such as protamine sulfate, disodium hydrogen phosphate, potassium hydrogen phosphate, sodium chloride, zinc salts, colloidal silica, magnesium trisilicate, polyvinyl pyrrolidone, cellulose-based substances, and PEG. Carriers for topical or gel-based forms of polypeptides include polysaccharides such as sodium carboxymethylcellulose or methylcellulose, polyvinylpyrrolidone, polyacrylates, polyoxyethylene-polyoxypropylene-block polymers, PEG, polymeric amino acids, amino acid copolymers, and lipid aggregates (such as oil droplets or liposomes).

The pharmaceutical compositions may also comprise pharmaceutically-acceptable, non-toxic carriers, excipients, stabilizers, or diluents, which are defined as vehicles commonly used to formulate pharmaceutical compositions for animal or human administration. The diluent is selected so as not to affect the biological activity of the combination. Acceptable carriers, excipients, or stabilizers are non-toxic to recipients at the dosages and concentrations employed, and include buffers such as phosphate, citrate, and other organic acids; antioxidants including ascorbic acid and methionine; preservatives (such as octadecyidimethylbenzyl ammonium chloride; hexamethonium chloride; benzalkonium chloride, benzethonium chloride; phenol, butyl or benzyl alcohol; alkyl parabens such as methyl or propyl paraben; catechol; resorcinol; cyclohexanol; 3-pentanol; and m-cresol); low molecular weight (less than about 10 residues) polypeptides; proteins, such as serum albumin, gelatin, or immunoglobulins; hydrophilic polymers such as polyvinylpyrrolidone; amino acids such as glycine, glutamine, asparagine, histidine, arginine, or lysine; monosaccharides, disaccharides, and other carbohydrates including glucose, mannose, or dextrins; chelating agents such as EDTA; sugars such as sucrose, mannitol, trehalose or sorbitol; salt-forming counter-ions such as sodium; metal complexes (e.g., Zn-protein complexes); and/or non-ionic surfactants such as TWEEN™, PLURONICS™ or polyethylene glycol (PEG).

Formulations to be used for in vivo administration are typically sterile. Sterilization of the compositions of the present disclosure may readily accomplished by filtration through sterile filtration membranes.

Typically, compositions are prepared as injectables, either as liquid solutions or suspensions; solid forms suitable for solution in, or suspension in, liquid vehicles prior to injection can also be prepared. The preparation also can be emulsified or encapsulated in liposomes or micro particles such as polylactide, polyglycolide, or copolymer for enhanced adjuvant effect, as discussed above (Langer, Science 249: 1527, 1990 and Hanes, Advanced Drug Delivery Reviews 28: 97-119, 1997). The agents of this disclosure can be administered in the form of a depot injection or implant preparation which can be formulated in such a manner as to permit a sustained or pulsatile release of the active ingredient. The pharmaceutical compositions are generally formulated as sterile, substantially isotonic and in full compliance with all Good Manufacturing Practice (GMP) regulations of the U.S. Food and Drug Administration.

Administration of a binding protein described herein may be achieved through any of a variety of art recognized methods including but not limited to the topical, intravascular injection (including intravenous or intraarterial infusion), intradermal injection, subcutaneous injection, intramuscular injection, intraperitoneal injection, intracranial injection, intratumoral injection, intranodal injection, transdermal, transmucosal, iontophoretic delivery, intralymphatic injection (Senti and Kundig (2009) Current Opinions in Allergy and Clinical Immunology 9(6):537-543), intragastric infusion, intraprostatic injection, intravesical infusion (e.g., bladder), respiratory inhalers including nebulizers, intraocular injection, intraabdominal injection, intralesional injection, intraovarian injection, intracerebral infusion or injection, intracerebroventricular injection (ICVI), and the like. In some embodiments, administration includes the administration of the binding protein itself (e.g., parenteral), as well as the administration of a recombinant vector (e.g., viral or non-viral vector) to cause the in situ expression of the binding protein in the subject. Alternatively, a cell, such as a cell isolated from the subject, could also be recombinantly modified to express the binding protein of the present disclosure.

The dosage of the pharmaceutical compositions depends on factors including the route of administration, the disease to be treated, and physical characteristics, e.g., age, weight, general health, of the subject. Typically, the amount of a binding protein contained within a single dose may be an amount that effectively prevents, delays, or treats the disease without inducing significant toxicity. A pharmaceutical composition of the disclosure may include a dosage of a binding protein described herein ranging from 0.01 to 500 mg/kg (e.g., from 0.01 to 450 mg, from 0.01 to 400 mg, from 0.01 to 350 mg, from 0.01 to 300 mg, from 0.01 to 250 mg, from 0.01 to 200 mg, from 0.01 to 150 mg, from 0.01 to 100 mg, from 0.01 to 50 mg, from 0.01 to 10 mg, from 0.01 to 1 mg, from 0.1 to 500 mg/kg, from 1 to 500 mg/kg, from 5 to 500 mg/kg, from 10 to 500 mg/kg, from 50 to 500 mg/kg, from 100 to 500 mg/kg, from 150 to 500 mg/kg, from 200 to 500 mg/kg, from 250 to 500 mg/kg, from 300 to 500 mg/kg, from 350 to 500 mg/kg, from 400 to 500 mg/kg, or from 450 to 500 mg/kg) and, in a more specific embodiment, about 1 to about 100 mg/kg (e.g., about 1 to about 90 mg/kg, about 1 to about 80 mg/kg, about 1 to about 70 mg/kg, about 1 to about 60 mg/kg, about 1 to about 50 mg/kg, about 1 to about 40 mg/kg, about 1 to about 30 mg/kg, about 1 to about 20 mg/kg, about 1 to about 10 mg/kg, about 10 to about 100 mg/kg, about 20 to about 100 mg/kg, about 30 to about 100 mg/kg, about 40 to about 100 mg/kg, about 50 to about 100 mg/kg, about 60 to about 100 mg/kg, about 70 to about 100 mg/kg, about 80 to about 100 mg/kg, or about 90 to about 100 mg/kg). In some embodiments, a pharmaceutical composition of the disclosure may include a dosage of a binding protein described herein ranging from 0.01 to 20 mg/kg (e.g., from 0.01 to 15 mg/kg, from 0.01 to 10 mg/kg, from 0.01 to 8 mg/kg, from 0.01 to 6 mg/kg, from 0.01 to 4 mg/kg, from 0.01 to 2 mg/kg, from 0.01 to 1 mg/kg, from 0.01 to 0.1 mg/kg, from 0.01 to 0.05 mg/kg, from 0.05 to 20 mg/kg, from 0.1 to 20 mg/kg, from 1 to 20 mg/kg, from 2 to 20 mg/kg, from 4 to 20 mg/kg, from 6 to 20 mg/kg, from 8 to 20 mg/kg, from 10 to 20 mg/kg, from 15 to 20 mg/kg). The dosage may be adapted by the physician in accordance with conventional factors such as the extent of the disease and different parameters of the subject.

A pharmaceutical composition containing a binding protein described herein can be administered to a subject in need thereof, for example, one or more times (e.g., 1-10 times or more) daily, weekly, monthly, biannually, annually, or as medically necessary. Dosages may be provided in either a single or multiple dosage regimens. The timing between administrations may decrease as the medical condition improves or increase as the health of the patient declines. A course of therapy may be a single dose or in multiple doses over a period of time. In some embodiments, a single dose is used. In some embodiments, two or more split doses administered over a period of 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 21, 28, 30, 60, 90, 120 or 180 days are used. Each dose administered in such split dosing protocols may be the same in each administration or may be different. Multi-day dosing protocols over time periods may be provided by the skilled artisan (e.g., physician) monitoring the administration, taking into account the response of the subject to the treatment including adverse effects of the treatment and their modulation as discussed above.

VIII. Indications

Neoplastic Diseases

The present disclosure provides methods of use of binding proteins in the treatment of subjects suffering from a neoplastic disease by the administration of a therapeutically effective amount of a binding protein (or nucleic acid encoding a binding protein including recombinant vectors encoding binding proteins) as described herein.

The compositions and methods of the present disclosure are useful in the treatment of subject suffering from a neoplastic disease characterized by the presence neoplasms, including benign and malignant neoplasms, and neoplastic disease. Examples benign neoplasms amenable to treatment using the compositions and methods of the present disclosure include but are not limited to adenomas, fibromas, hemangiomas, and lipomas. Examples of pre-malignant neoplasms amenable to treatment using the compositions and methods of the present disclosure include but are not limited to hyperplasia, atypia, metaplasia, and dysplasia. Examples of malignant neoplasms amenable to treatment using the compositions and methods of the present disclosure include but are not limited to carcinomas (cancers arising from epithelial tissues such as the skin or tissues that line internal organs), leukemias, lymphomas, and sarcomas typically derived from bone fat, muscle, blood vessels or connective tissues). Also included in the term neoplasms are viral induced neoplasms such as warts and EBV induced disease (i.e., infectious mononucleosis), scar formation, hyperproliferative vascular disease including intimal smooth muscle cell hyperplasia, restenosis, and vascular occlusion and the like.

The term “neoplastic disease” includes cancers characterized by solid tumors and non-solid tumors including but not limited to breast cancers; sarcomas (including but not limited to osteosarcomas and angiosarcomas and fibrosarcomas), leukemias, lymphomas, genitourinary cancers (including but not limited to ovarian, urethral, bladder, and prostate cancers); gastrointestinal cancers (including but not limited to colon esophageal and stomach cancers); lung cancers; myelomas; pancreatic cancers; liver cancers; kidney cancers; endocrine cancers; skin cancers; and brain or central and peripheral nervous (CNS) system tumors, malignant or benign, including gliomas and neuroblastomas, astrocytomas, myelodysplastic disorders; cervical carcinoma-in-situ; intestinal polyposes; oral leukoplakias; histiocytoses, hyperprofroliferative scars including keloid scars, hemangiomas; hyperproliferative arterial stenosis, psoriasis, inflammatory arthritis; hyperkeratoses and papulosquamous eruptions including arthritis.

The term neoplastic disease includes carcinomas. The term “carcinoma” refers to malignancies of epithelial or endocrine tissues including respiratory system carcinomas, gastrointestinal system carcinomas, genitourinary system carcinomas, testicular carcinomas, breast carcinomas, prostatic carcinomas, endocrine system carcinomas, and melanomas. The term neoplastic disease includes adenocarcinomas. An “adenocarcinoma” refers to a carcinoma derived from glandular tissue or in which the tumor cells form recognizable glandular structures.

The term “hematopoietic neoplastic disorders” refers to neoplastic diseases involving hyperplastic/neoplastic cells of hematopoietic origin, e.g., arising from myeloid, lymphoid or erythroid lineages, or precursor cells thereof. Myeloid neoplasms include, but are not limited to, myeloproliferative neoplasms, myeloid and lymphoid disorders with eosinophilia, myeloproliferative/myelodysplastic neoplasms, myelodysplastic syndromes, acute myeloid leukemia and related precursor neoplasms, and acute leukemia of ambiguous lineage. Exemplary myeloid disorders amenable to treatment in accordance with the present disclosure include, but are not limited to, acute promyeloid leukemia (APML), acute myelogenous leukemia (AML) and chronic myelogenous leukemia (CML). Lymphoid neoplasms include, but are not limited to, precursor lymphoid neoplasms, mature B-cell neoplasms, mature T-cell neoplasms, Hodgkin's Lymphoma, and immunodeficiency-associated lymphoproliferative disorders. Exemplary lymphic disorders amenable to treatment in accordance with the present disclosure include, but are not limited to, acute lymphoblastic leukemia (ALL) which includes B-lineage ALL and T-lineage ALL, chronic lymphocytic leukemia (CLL), prolymphocytic leukemia (PLL), hairy cell leukemia (HLL) and Waldenstrom's macroglobulinemia (WM).

In some instances, the hematopoietic neoplastic disorder arises from poorly differentiated acute leukemias (e.g., erythroblastic leukemia and acute megakaryoblastic leukemia). As used herein, the term “hematopoietic neoplastic disorders” refers malignant lymphomas including, but are not limited to, non-Hodgkins lymphoma and variants thereof, peripheral T cell lymphomas, adult T-cell leukemia/lymphoma (ATL), cutaneous T cell lymphoma (CTCL), large granular lymphocytic leukemia (LGF), Hodgkin's disease and Reed-Steinberg disease.

The determination of whether a subject is “suffering from a neoplastic disease” refers to a determination made by a physician with respect to a subject based on the available information accepted in the field for the identification of a disease, disorder or condition including but not limited to X-ray, CT-scans, conventional laboratory diagnostic tests (e.g., blood count, etc.), genomic data, protein expression data, immunohistochemistry, that the subject requires or will benefit from treatment.

The determination of efficacy of the methods of the present disclosure in the treatment of cancer is generally associated with the achievement of one or more art recognized parameters such as reduction in lesions particularly reduction of metastatic lesion, reduction in metastatsis, reduction in tumor volume, improvement in ECOG score, and the like. Determining response to treatment can be assessed through the measurement of biomarker that can provide reproducible information useful in any aspect of binding protein therapy, including the existence and extent of a subject's response to such therapy and the existence and extent of untoward effects caused by such therapy. The response to treatment may be characterized by improvements in conventional measures of clinical efficacy may be employed such as Complete Response (CR), Partial Response (PR), Stable Disease (SD) and with respect to target lesions, Complete Response (CR),” Incomplete Response/Stable Disease (SD) as defined by RECIST as well as immune-related Complete Response (irCR), immune-related Partial Response (irPR), and immune-related Stable Disease (irSD) as defined Immune-Related Response Criteria (irRC) are considered by those of skill in the art as evidencing efficacy in the treatment of neoplastic disease in mammalian (e.g., human) subjects.

Infectious Diseases

The present disclosure provides methods of use of binding proteins in the treatment of subjects suffering from an infectious disease by the administration of a therapeutically effective amount of a binding protein (or nucleic acid encoding an binding protein including recombinant vectors encoding binding proteins) as described herein.

In some embodiments the infection is a chronic infection, i.e., an infection that is not cleared by the host immune system within a period of up to 1 week, 2 weeks, etc. In some cases, chronic infections involve integration of pathogen genetic elements into the host genome, e.g., retroviruses, lentiviruses, Hepatitis B virus, etc. In other cases, chronic infections, for example certain intracellular bacteria or protozoan pathogens, result from a pathogen cell residing within a host cell. Additionally, in some embodiments, the infection is in a latent stage, as with herpes viruses or human papilloma viruses.

Viral pathogens of interest include without limitation, retroviral, hepadna, lentiviral, etc. pathogens, e.g., HIV-1; HIV-2, HTLV, FIV, SIV, etc., Hepatitis A, B, C, D, E virus, etc. In some embodiments, the methods of the invention involve diagnosis of a patient as suffering from an infection; or selection of a patient previously diagnosed as suffering from an infection; treating the patient with a regimen of variant type III interferon therapy, optionally in combination with an additional therapy; and monitoring the patient for efficacy of treatment. Monitoring may measure clinical indicia of infection, e.g., fever, white blood cell count, etc., and/or direct monitoring for presence of the pathogen. Treatment may be combined with other active agents. Cytokines may also be included, e.g., interferon γ, tumor necrosis factor α, interleukin 12, etc. Antiviral agents, e.g., acyclovir, gancyclovir, etc., may also be used in treatment. Subjects suspected of having an infection, including an HCV infection, can be screened prior to therapy. Further, subjects receiving therapy may be tested in order to assay the activity and efficacy of the treatment. Significant improvements in one or more parameters is indicative of efficacy. It is well within the skill of the ordinary healthcare worker (e.g., clinician) to adjust dosage regimen and dose amounts to provide for optimal benefit to the patient according to a variety of factors (e.g., patient-dependent factors such as the severity of the disease and the like, the compound administered, and the like). For example, HCV infection in an individual can be detected and/or monitored by the presence of HCV RNA in blood, and/or having anti-HCV antibody in their serum. Other clinical signs and symptoms that can be useful in diagnosis and/or monitoring of therapy include assessment of liver function and assessment of liver fibrosis (e.g., which may accompany chronic viral infection).

Subjects for whom the therapy described herein can be administered include naïve individuals (e.g., individuals who are diagnosed with an infection, but who have not been previously treated) and individuals who have failed prior treatment (“treatment failure” patients). For HCV therapy, previous treatment includes, for example, treatment with IFN-α monotherapy (e.g., IFN-α and/or PEGylated IFN-α) or IFN-α combination therapy, where the combination therapy may include administration of IFN-α and an antiviral agent such as ribavirin. Treatment failure patients include non-responders (i.e., individuals in whom the HCV titer was not significantly or sufficiently reduced by a previous treatment for HCV to provide a clinically significant response, e.g., a previous IFN-α monotherapy, a previous IFN-α and ribavirin combination therapy, or a previous pegylated IFN-α and ribavirin combination therapy); and relapsers (i.e., individuals who were previously treated for HCV (e.g., who received a previous IFN-α monotherapy, a previous IFN-α and ribavirin combination therapy, or a previous pegylated IFN-α and ribavirin combination therapy), in whom the HCV titer decreased to provide a clinically significant response, but in whom the decreased HCV titer was not maintained due to a subsequent increase in HCV titer).

Other subjects for whom the therapy disclosed herein is of interest include subject who are“difficult to treat” subjects due to the nature of the HCV infection. “Difficult to treat” subjects are those who 1) have high-titer HCV infection, which is normally defined as an HCV titer of at least about 10⁵, at least about 5×10⁵, or at least about 10⁶or more genome copies of HCV per milliliter of serum, 2) are infected with HCV of a genotype that is recognized in the field as being associated with treatment failure (e.g., HCV genotype 1, subtypes thereof (e.g., 1a, 1b, etc.), and quasispecies thereof or 3) both.

In other embodiment methods are provided for treating or reducing primary or metastatic cancer in a regimen comprising contacting a subject in need of treatment with a therapeutically effective amount or an effective dose of IFN λ synthekines or IFN λ variant polypeptides. Effective doses for the treatment of cancer vary depending upon many different factors, including means of administration, target site, physiological state of the patient, whether the patient is human or an animal, other medications administered, and whether treatment is prophylactic or therapeutic. Usually, the patient is a human, but nonhuman mammals may also be treated, e.g., companion animals such as dogs, cats, horses, etc., laboratory mammals such as rabbits, mice, rats, etc., and the like. Treatment dosages can be titrated to optimize safety and efficacy.

In prophylactic applications, a relatively low dosage may be administered at relatively infrequent intervals over a long period of time. Some patients continue to receive treatment for the rest of their lives. In other therapeutic applications, a relatively high dosage at relatively short intervals is sometimes required until progression of the disease is reduced or terminated, and preferably until the patient shows partial or complete amelioration of symptoms of disease. Thereafter, the patent can be administered a prophylactic regime.

In still other embodiments, methods of the present invention include treating, reducing or preventing tumor growth, tumor metastasis or tumor invasion of cancers including carcinomas, hematologic cancers, melanomas, sarcomas, gliomas, particularly cancers of epithelial origin that express IFN λR1 and IFNAR1 or IFNAR2, or IL-10Rβ and IFNAR1 or IFNAR2. In some embodiments a cancer is assessed for responsiveness to an IFN λ synthekine by determining whether the cancer expresses the cognate receptors that the synthekine activates, e.g., determining the expression of IFN λR1, and IFNAR1 or IFNAR2. Tissues known to express IFN λR1 include, for example, lung, heart, liver (hepatocytes), prostate, keratinocytes and melanocytes. Cancers responsive to IFN λ and IFN λ synthekines may include, without limitation, melanoma, fibrosarcoma, hepatocellular carcinoma, bladder carcinoma, Burkitt's lymphoma, colorectal carcinoma, glioblastoma, non-small cell lung cancer, esophageal carcinoma, and osteosarcoma, among others.

For prophylactic applications, pharmaceutical compositions or medicaments are administered to a patient susceptible to, or otherwise at risk of disease in an amount sufficient to eliminate or reduce the risk, lessen the severity, or delay the outset of the disease, including biochemical, histologic and/or behavioral symptoms of the disease, its complications and intermediate pathological phenotypes presenting during development of the disease.

EXAMPLES

Example 1—V_hH Generation

Camels were acclimated at research facility for at least 7 days before immunization. Antigen was diluted with 1×PBS (antigen total about 1 mg). The quality of the antigen was assessed by SDS-PAGE to ensure purity (e.g., >80%). For the first time, 10 mL CFA (then followed 6 times using IFA) was added into mortar, then 10 mL antigen in 1×PBS was slowly added into the mortar with the pestle grinding. The antigen and CFA/IFA were ground until the component showed milky white color and appeared hard to disperse. Camels were injected with antigen emulsified in CFA subcutaneously at at least six sites on the body, injecting about 2 mL at each site (total of 10 mL per camel). A stronger immune response was generated by injecting more sites and in larger volumes. The immunization was conducted every week (7 days), for 7 times. The needle was inserted into the subcutaneous space for 10 to 15 seconds after each injection to avoid leakage of the emulsion. Alternatively, a light pull on the syringe plunger also prevented leakage. The blood sample was collected three days later after 7^thimmunization.

After immunization, the library was constructed. Briefly, RNA was extracted from blood and transcribed to cDNA. The V_HH regions were obtained via two-step PCR, which fragment about 400 bp. The PCR outcomes and the vector of pMECS phagemid were digested with Pst I and Not I, subsequently, ligated to pMECS/Nb recombinant. After ligation, the products were transformed into Escherichia coli (E. coli) TG1 cells by electroporation. Then, the transformants were enriched in growth medium and planted on plates. Finally, the library size was estimated by counting the number of colonies.

Library biopanning was conducted to screen candidates against the antigens after library construction. Phage display technology was applied in this procedure. Positive colonies were identified by PE-ELISA.

Example 2. Generation of Anti-hIL10R VHHs

Camels were immunized with the extracellular domains of the human IL10Rα (amino acids 22-235, UniProtKB Q13651, hIL-10Rα_ecd) and IL10Rβ (amino acids 20-220, UniProtKB Q08334, hIL-10β_ecd) weekly for seven weeks and PBMCs harvested on day 52. Phage display libraries were constructed and biopanning conducted as described in Example 1 above. 50 VHH sequences were obtained after selection on hIL10-R1 and 47 VHH sequences were obtained after selection on hIL10-R2. Sequences were clonotyped using germline assignment and CDR3 sequence similarity.

Example 3. Synthesis of DNA Encoding Synthekines

Seven unique anti-hIL-10Rα_ecdsequences (SEQ ID Nos: 44-50) and seven unique anti-hIL-10Rβ_ecdsequences (SEQ ID Nos: 51-57) were selected from each cohort and DNA was synthesized consisting of one IL-10Rα VHH encoding DNA and one IL-10Rβ VHH encoding DNA separated by a linker sequence by GGGS (SEQ ID NO:23) encoding DNA. DNA was for each possible VHH combination and in both orientations for a total of 98 7×7×2=98 VHH dimers. An Ala-Ser (“AS”) linker followed by His-6 (SEQ ID NO: 442) DNA (ASH6, SEQ ID NO: 430) was added at the 3′ end of each DNA construct. The codon optimized DNA sequences encoding these constructs are provided as SEQ ID Nos: 290-237 and the orientation of components thereof are described in Table 2 of the specification above.

Example 4. Recombinant Production and Purification

Codon optimized DNA inserts (SEQ ID Nos: 290-237) and cloned into modified pcDNA3.4 (Genscript) for small scale expression in HEK293 cells in 24 well plates. Supernatants The cells The IL2R binding proteins were purified in substantial accordance with the following procedure. Using a Hamilton Star automated system, 96×4 ml of supernatants in 4×24-well blocks were re-arrayed into 4×96-well, 1 mL blocks. PhyNexus micropipette tips (Biotage, San Jose CA) holding 80 uL of Ni-Excel IMAC resin (Cytiva) are equilibrated wash buffer: PBS pH 7.4, 30 mM imidazole. PhyNexus tips were dipped and cycled through 14 cycles of 1 mL pipetting across all 4×96-well blocks. PhyNexus tips were washed in 2×1 mL blocks holding wash buffer. PhyNexus tips were eluted in 3×0.36 mL blocks holding elution buffer: PBS pH 7.4, 400 mM Imidazole. PhyNexus tips were regenerated in 3×1 mL blocks of 0.5 M sodium hydroxide.

The purified protein eluates were quantified using a Biacore® T200 as in substantial accordance with the following procedure. 10 uL of the first 96×0.36 mL eluates were transferred to a Biacore® 96-well microplate and diluted to 60 uL in HBS-EP+ buffer (10 mM Hepes pH 7.4, 150 mM NaCl, 1 mM EDTA, 0.05% Tween 20). Each of the 96 samples was injected on a CM5 series S chip previously functionalized with anti-histidine capture antibody (Cytiva): injection is performed for 18 seconds at 5 uL/min. Capture levels were recorded 60 seconds after buffer wash. A standard curve of known VHH concentrations (270, 90, 30, 10, 3.3, 1.1 μg/mL) was acquired in each of the 4 Biacore chip flow cells to eliminate cell-to-cell surface variability. The 96 captures were interpolated against the standard curve using a non-linear model including specific and unspecific, one-site binding. Concentrations in the first elution block varied from 12 to 452 μg/mL corresponding to a 4-149 μg. SDS-PAGE analysis of 5 randomly picked samples was performed to ensure molecular weight of eluates corresponded to expected values (˜30 KDa).

The concentration of the proteins was normalized using the Hamilton Star automated system in substantial accordance with the following procedure. Concentration values are imported in an Excel spreadsheet where pipetting volumes were calculated to perform dilution to 50 μg/mL in 0.22 mL. The spreadsheet was imported in a Hamilton Star method dedicated to performing dilution pipetting using the first elution block and elution buffer as diluent. The final, normalized plate was sterile filtered using 0.22 μm filter plates (Corning) and the material used for the following in vitro assays.

Example 5. IL10 Activity Assay

HEK-Blue™ IL-10 reporter cell line (Invivogen, San Diego CA) was used for screening the IL10R1/R2 VHHs. HEK-Blue™ IL-10 cells were generated by stable transfection of the human embryonic kidney HEK293 cell line with the genes encoding hIL-10Rα and R chains, human STAT3, and the STAT3-inducible SEAP (secreted embryonic alkaline phosphatase) reporter. Binding of IL-10 to its receptor on the surface of HEK-Blue™ IL-10 cells triggers JAK1/STAT3 signaling and the subsequent production of SEAP. The signal was then detected by quantifying SEAP activity in the cell culture supernatant using a QUANTI-Blue™ development solution (Invivogen, San Diego CA) and the absorbance values were measured spectrophotometrically at 630 nm. Because STAT3 is also implicated in the signaling of cytokines such as IFN-α/β and IL-6, HEK-Blue™ IL-10 cells are knockout for the expression of hIFNAR2 and hIL-6R.

Example 6. Screening of SEQ ID NOs: 192-289

To screen the IL10R1/R2 VHHs, HEK-Blue™ IL-10 cells were seeded in a 96-well plate at 50,000 cells per well and treated with either 25 nM or 100 nM protein (in triplicates) for 24 hours. Recombinant Animal-Free Human IL-10 (Shenandoah Biotechnology, Inc. Warwick, PA Catalog No. 100-83AF) was used as a positive control and unstimulated cells were used as a negative control. 24 hours post treatment, 20 μl of the cell supernatant was transferred to a flat-bottom 96 well plate and the assay was developed by adding 180 μl of the QUANTI-Blue™ (Invivogen) for 2 hours. The absorbance values were measured at 630 nm on the Envision® (PerkinElmer, Waltham MA) multilabel plate reader. The results of this screening are presented in Table 3 of the specification.

INFORMAL SEQUENCE LISTING

SEQ
ID
NO	Notes	Amino Acid or DNA Sequence

1	linker	GGGGS

2	linker	GGGGGS

3	linker	GGSG

4	linker	SGGG

5	linker	GSGS

6	linker	GSGSGS

7	linker	GSGSGSGSGS

8	linker	GSGSGSGSGSGS

9	linker	GGSGGS

10	linker	GGSGGSGGS

11	linker	GGSGGSGGSGGS

12	linker	GGSGGGSG

13	linker	GGSGGGSGGGSG

14	linker	GGSGGGSGGGSGGGSG

15	linker	GGSGGGSGGGSGGGSGGGSG

16	linker	GGGGSGGGGS

17	linker	GGGGSGGGGSGGGGS

18	linker	GGSGG

19	linker	GSGSG

20	linker	GSGGG

21	linker	GGGSG

22	linker	GSSSG

23	linker	GGGS

24	Anti-gp130 V_HH	VAAIWPGGGLTVYADSVKGRFTISRDHAKNTLYLQ
		MNNLKPEDTAMYYCAAQVQLQESGGGSVQAGGSLR
		LSCTASGAIASGYIDSRWCMAWFRQAPGKEREGGS
		PRMCPSLEFGFDYWGQGTQVTVSS

25	Anti-gp130 V_HH	SDGTTRYADSVKGRFTISQGTAKNTVYLQMNSLQP
		EDTAMYYCKTVCVVGSRQVQLQESGGGSVQAGGSL
		RLSCVASASTYCTYDMHWYRQAPGKGREFVSAIDW
		SDYWGQGTQVTVSS

26	Anti-gp130 V_HH	DGTTGYADSVKGRFTISKDKAKDTVYLQMNSLKPE
		DTGMYSCKTKDGTIATMQVQLQESGGGSVQAGGSL
		RLSCTAPGFTSNSCGMDWYRQAPGKEREFVSSIST
		ELCDFGYWGQGTQVTVSS

27	Anti-gp130 V_HH	TGDGRTYYADSVKGRFTISRDNAKNTVDLQMSSLK
		PEDTAMYYCAARAAPLYQVQLQESGGGSVQAGGSL
		RLSCAASGYPYSNGYMGWFRQAPGKEREGVATIYS
		SGSPLTRARYNVWGQGTQVTVSS

28	Anti-gp130 V_HH	SDGSTYYADSVKGRFTITRDNAKNTVYLQMNSLKP
		EDTAIYYCSANCYRRLRNQVQLQESGGGSVQAGGS
		LTLSCAASEYAYSTCNMGWYRQAPGKERELVSAFI
		YWGQGTQVTVSS

29	Anti-gp130 V_HH	SGANAFYADSVKGRFTISRDNAKNTLYLQMNSLKP
		EDTATYYCKRGHACAGYQVQLQESGGGLVQPGGSL
		RLSCTASGLTFDDSVMGWFRQAPGKGREAVSCISS
		YPIPYDDYWGQGTQVTVSS

30	Anti-I12Rb/Anti-	QVQLQESGGGSVQAGGSLRLSCAASGYEYCRIHMT
	CD122 V_HH	WYRQGPGKEREFVSSIGSDGRKTYANSVTGRFTIS
		RDNANHTVYLQMNSLSPEDTAMYYCKTEYLYGLGC
		PDGSAYWGQGTQVTVSS

31	Anti-I12Rb/Anti-	QVQLQESGGGSVQAGGSLRLSCAASEYTASRYCMA
	CD 122 V_HH	WFRQAPGKEREGVAAIHPGGGTTYYADSVKGRFSI
		SQDSADNTLYLQMNSLKPEDTAMYYCAAGSLWVPF
		GDRCAANYWGQGTQVTVSS

32	Anti-I12Rb/Anti-	QVQLQESGGGLVQPGGSLRLSCVASGFTFSNYWIF
	CD122 V_HH	WVRQAAGKGLEWLSTSNTGGDTTKYADSVKGRFTI
		SRDSAKNTEYLQMNSLKPEDTAVYYCETGRCARSG
		GYQGTQVTVSS

33	Anti-I12Rb/Anti-	QVQLQESGGGSVQVGGSLRLSCATSGDTKSIRCMG
	CD122 V_HH	WFRQTPGKEREGIAAIDREGFATYADSVYDRFTIA
		QDNAQNTLYLEMNALKPEDTAMYYCAAQNMCRVVR
		GAMTGVDYWGKGTQVTVSS

34	Anti-I12Rb/Anti-	QVQLQESGGGSVQVGGSLKLSCAASGYTYSSYYCM
	CD122 V_HH	GWFRQAPGKEREGVAAIDSDGSTSYADSVKGRFTI
		SQDDAKNTLYLQMNSLKPEDTAMYYCAASYEVVDC
		YPSGYGQDYWGKGTQVTVSS

35	Anti-I12Rb/Anti-	QVQLQESGGGSVQAGGSLRLSCVGSGYTYDTSDMS
	CD122 V_HH	WYRQAPGKEREFVSDIDSGDWAAYADAVKGRFTIS
		RDNAKKTVYLQMNSLEPEDTAMYYCKASYWKWGKL
		NNFWGPGTQVTVSS

36	Anti-I12Rb/Anti-	QVQLQESGGGLVQPGGSLKLSCAASGFRFSNYGMS
	CD122 V_HH	WVRQAPGEGLEWVSYINGDGSRTHYADSVKGRFTI
		SRDNAKNTLYLQLNSLKTEDTAMYYCEKGLSRDGW
		SLSAASRGQGTQVTVSS

37	Anti-I12Rb/Anti-	QVQLQESGGGSVQTGGSLRLSCAVSGYTTYSFNYM
	CD122 V_HH	GWFRQAPGKEREGVAVIYTGGGSTLYADSVKGRFT
		ISQDNAKNTVYLQMNSLKPEDTAMYYCAADDQRFA
		SPLYAYFGYWGQGTQVTVSS

38	Anti- IL2Rgamma/	DGGSTAYAASVEGRFTISRDNAKSTLYLQLNSLKT
	Anti-CD132	EDTAMYYCTKGYGDGTPQVQLQESGGGLVQPGGSL
		RLSCTASGFSFSSYPMTWARQAPGKGLEWVSTIAS
		APGQGTQVTVSS

39	Anti- IL2Rgamma/	GGGTFYADSVKGRFTISRDNAKNTLYLQLNSLKAE
	Anti-CD132	DTAMYYCATNRLHYYSDQVQLQESGGGLVQPGGSL
		RLSCAASGFTFSSAHMSWVRQAPGKGREWIASIYS
		DDSLRGQGTQVTVSS

40	Anti- IL2Rgamma/	DGSTYYADSVKGRFTISQDNAKNTVYLQMDSVKPE
	Anti-CD132	DTAVYYCAADFMIAIQAQVQLQESGGGSVQAGGSL
		RLSCTASGFTFDDREMNWYRQAPGNECELVSTISS
		PGAGCWGQGTQVTVSS

41	Anti- IL2Rgamma/	RSIYYADSVKGRFTISQDNAKNTLYLQMNSLKPED
	Anti-CD132	IAMYSCAAGGYSWSAGCEQVQLQESGGGSVQAGGS
		LRLSCVASGYTSCMGWFRQAPGKEREAVATIYTRG
		FNYWGQGTQVTVSS

42	Anti- IL2Rgamma/	DGSTYYADSVKGRFTISQDNAKNTVYLQMNSLKPE
	Anti-CD132	DTAVYYCAAEPRGYYSNQVQLQESGGGSVQAGGSL
		RLSCTASGFTFDDSDMGWYRQAPGNECELVSTISS
		YGGRRECNYWGQGTQVTVSS

43	Anti- IL2Rgamma/	GGSTYYADSVKGRFTISQDNAKNTLYLQMNSLKPE
	Anti-CD132	DTAMYYCAAAWVACLEQVQLQESGGGSVQAGGSLR
		LSCVASGYTFSSYCMGWFRQAPGKEREGVAALGFG
		GSWYDLARYKHWGQGTQVTVSS

44	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMA
		WFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTI
		SQDNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSY
		LFDAQSFTYWGQGTQVTVSS

45	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMG
		WFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVP
		GFCGFLLSAGMDYWGKGTQVTVSS

46	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMG
		WFRQAPGKEREGVAQINSDGSTSYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGS
		WYERLCGPYTYEYNYWGQGTQVTVSS

47	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMG
		WFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTIS
		KDNAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGG
		SCLFLGPEIKVSKADFRYWGQGTQVTVSS

48	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMG
		WFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTI
		SQDNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVY
		GGSCPTPTFDYWGQGTQVTVSS

49	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMG
		WFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTIS
		KDNGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPP
		CGVLYLGMDYWGKGTQVTVSS

50	Anti-IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMT
		WYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFIS
		QDNAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAH
		GGSWYSVRANYWGQGTQVTVSS

51	Anti-IL10Rβ	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
		SGCMGWFRQAPGKEREAVAAINSDGSTSYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
		QVTVSS

52	Anti-IL10Rβ	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
		SYCMGWFRQAPGKEREGVAHIDSDGSTSYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCAADPIPGPGYCDGGPNKYWGQGTQV
		TVSS

53	Anti-IL10Rβ	QVQLQESGGGSVQAGGSLRLSCAASRYTYN
		SYCMGWFRQAPGKEREGVATIDSDGMTRYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCAADADCTIAAMTTNPLGQGTQVTVS
		S

54	Anti-IL10Rβ	QVQLQESGGGSVQAGGSLRLSCTVSRYTAS
		VNYMGWFRQAPGKEREGVATIFTGAGTTYY
		ANSVKGRFTISRDNAKNTAYLQMNSLKPED
		TAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
		VTVSS

55	Anti-IL10Rβ	QVQLQESGGGSVEAGGSLRLSCAASGYTHS
		SYCMGWFRQAPGKEREGVAAIDVDGSTTYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		GMYYCAAEFADCSSNYFLPPGAVRYWGQGT
		QVTVSS

56	Anti-IL10Rβ	QVQLQESGGGSVQAGGSLRLSCAASGYSYS
		SYCMGWFRQAPGKEREGVATIDSDGMTRYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
		TVSS

57	Anti-IL10Rβ	QVQLQESGGGSVQTGGSLRLSCAASGYTYL
		RGCMGWFRQAPGKEREGVAVMDVVGDRRSY
		IDSVKGRFTISRDNAANSVYLQMDNLKPED
		TAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
		SS

58	Anti-IL12Rβ2	QVQLQESGGGSVQAGGSLRLSCAASGFTVT
		RYCMGWLRQAPGKQREGVAIIERDGRTGYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCGAIEGSCRPDFGYRGQGTQVTVSS

59	Anti-IL12Rβ2	QVQLQESGGGSVQAGGSLRLSCTASGLTFD
		DVEMAWYRQGPGDDYDLVSSINTDSRVYYV
		DSVKDRFTISRDNAKNTLYLQMNNLKPEDT
		AVYYCAADPWGGDLRGYPNYWGQGTQVTVS
		S

60	Anti-IL12Rβ2	QVQLQESGGGLVQAGGSLRLSCQASGYTYG
		LFCMGWFRQVSGKKREGVAVVDSPGGRHVA
		DSLKGRFTISKDNANNILYLDMTNLKSEDT
		ATYYCAADPEKYCFLFSDAGYQYWGQGTQV
		TVSS

61	Anti-IL12Rβ2	QVQLQESGGGSVQAGGSLRLSCAASGVTYS
		RYCMGWFRQAPGLERERVAHIYSRGIITYY
		TDSVKGRFTISQDSAKKTVYLQMNSLKPED
		TAMYYCAATRETYGGSGDCGYESVYNYWAQ
		GTQVTVSS

62	Anti-IL12Rβ2	QVQLQESGGGLVQPGGSLKLSCAASGFTFS
		TYAMSWVRQAPGKEPEWISRISSGGGNTYY
		ADAVKGRFAISRDNAKNTLYLQLNSLKTED
		TAIYVCTMDDYYGGSWHPISRGHGTQVTVS
		S

63	Anti-IL12Rβ2	QVQLQESGGGSVQAGGSLRLSCSASGFTVD
		DFAMGWYRQAPGNECELVSTISSGGSTYYA
		DSVKGRFTISQDSAKNTVYLQMNSLKPEDT
		AVYYCAPSSVGCPLGYWGQGTQVTVSS

64	Anti-IL23R	QVQLQESGGGSVQAGGSLRLSCAASGFTVT
		RYCMGWLRQAPGKQREGVAIIERDGRTGYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCGAIEGSCRPDFGYRGQGTQVTVSS

65	Anti-IL23R	QVQLQESGGGSVQAGGSLRLSCTASGLTFD
		DVEMAWYRQGPGDDYDLVSSINTDSRVYYV
		DSVKDRFTISRDNAKNTLYLQMNNLKPEDT
		AVYYCAADPWGGDLRGYPNYWGQGTQVTVS
		S

66	Anti-IL23R	QVQLQESGGGLVQAGGSLRLSCQASGYTYG
		LFCMGWFRQVSGKKREGVAVVDSPGGRHVA
		DSLKGRFTISKDNANNILYLDMTNLKSEDT
		ATYYCAADPEKYCFLFSDAGYQYWGQGTQV
		TVSS

67	Anti-IL23R	QVQLQESGGGSVQAGGSLRLSCAASGVTYS
		RYCMGWFRQAPGLERERVAHIYSRGIITYY
		TDSVKGRFTISQDSAKKTVYLQMNSLKPED
		TAMYYCAATRETYGGSGDCGYESVYNYWAQ
		GTQVTVSS

68	Anti-IL23R	QVQLQESGGGLVQPGGSLKLSCAASGFTFS
		TYAMSWVRQAPGKEPEWISRISSGGGNTYY
		ADAVKGRFAISRDNAKNTLYLQLNSLKTED
		TAIYVCTMDDYYGGSWHPISRGHGTQVTVS
		S

69	Anti-IL23R	QVQLQESGGGSVQAGGSLRLSCSASGFTVD
		DFAMGWYRQAPGNECELVSTISSGGSTYYA
		DSVKGRFTISQDSAKNTVYLQMNSLKPEDT
		AVYYCAPSSVGCPLGYWGQGTQVTVSS

70	Anti-IL27Ralpha	VAYGITSYADSVKGRFTISRDNTKNTLYLQ
		LNSLKTEDTAIYYCVKHSGTTIPRQVQLQE
		SGGGLVQPGESLRLSCTASGFTFSNYAMSW
		VRQAPGKGLEWVSGINGFISYTKRGQGTQV
		TVSS

71	Anti-IL27Ralpha	GGDTTLYADSVKGRFTSSRDNAKNTLYLQL
		NSLKTEDTAIYYCAKRIDCNSGYQVQLQES
		GGGSVQVGGSLRLSCAASGFTFSSYPMSWV
		RQAPGKGLEWISTISACYRRNYWGQGTQVT
		VSS

72	Anti-IL27Ralpha	WVGGMLYFADSVKGRFTVSQDQAKNTLYLQ
		MNSLKPEDTAMYYCAAESVSSQVQLQESGG
		GSVQAGGSLRLSCRASGSTYSNYCLGWFRQ
		ITGKEREGVAVINFSCGGWLTRPDRVPYWG
		QGTQVTVSS

73	Anti-IL27Ralpha	GTGSTSYAASVKGRFTASQDKGKNIAYLQM
		NSLKPEDTAMYYCKASCVRGRGQVQLQESG
		GGSVQAGGSLRLSCVASGYVSCDYFLPSWY
		RQAPGKEREFVSIIDISEYWGQGTQVTVSS

74	Anti-IL27Ralpha	IYTVGGSIFYADSVRGRFTISQDATKNMFY
		LQMNTLKPEDTAMYYCAAASGRLQVQLQES
		GGGSVQSGGSLRLSCAASGFTYSTSNSWMA
		WFRQAPGKEREGVAARGKWFWPYEYNYWGQ
		GTQVTVSS

75	Anti-IL27Ralpha	GGASTYYTDSVKGRFTISRDNAKNMLYLQL
		NSLKTEDTAMYYCAKGGSGYGDQVQLQESG
		GGLVQPGGSLRLSCAASGFTFSHSGMSWVR
		QAPGKGLEWVSTINSASRMTSPGSQGTQVT
		VSS

76	Anti-IL28Ralpha	DGSTSYADSVKGRFTISKDNAKNTLYLQMN
		SLRPEDTAMYYCAADGEYNDYVQVQLQESG
		GGSVQSGGSLRLSCAASGFTYSSYCMGWFR
		QAPGKEREGVAAIDSCWSTGLRYRGQGTQV
		TVSS

77	Anti-IL28Ralpha	RDGSTFYPDSVKGRFTISRDNAKNTLYLQL
		NSLKTEDTAMYYCAKEEPGSSSRQVQLQES
		GGGLVQPGGSLRLSCVASGFTFSDYAMSWV
		RQAPGMGLERVSAIGGQGTQVTVSS

78	Anti-IL28Ralpha	SDGTTSYADSVKERFTISKDNAKNILYLQM
		NSLKPEDTARYYCAATALLLGRGQVQLQES
		GGGSVQAGGSLRLSCAVSRYTISRSDCMGW
		FRQAPGKEREGVARIGSACHKEVSVFSWWG
		QGTQVTVSS

79	Anti-IL28Ralpha	SGGDDTFYTDSVKGRFTISRDNAKNTLYLQ
		MNSLKTEDTAMYYCAMGASGMIQVQLQESG
		GGLVQPGGSLRLSCAASGFTFSNYGMSWVR
		QAPGKGLEWVSGINPRGQGTQITVSS

80	Anti-IL28Ralpha	TSGGAVVYADSVKGRFTISQDDAKNTMYLQ
		MNSLKPEDTAMYYCAASRAPAPQVQLQESG
		GGSVQLGGSLRLSCLVSGSTDNIKYMGWFR
		QAPGKEREGVAAVYPRLLLQRALVEYWGQG
		TQVTVSS

81	Anti-IL28Ralpha	QVQLQESGGGLVQPGGSLRLSCAASGFTFS
		NATMSWVRQAPGKEIEWVSAISNSRGTKYY
		AAFVKGRFTISRDNAKNTLYLQLNNLKTED
		TAMYYCTKDWKTSYSDYDLSDGQGTQVTVS
		S

82	Anti-IL28Ralpha	RDGKTYYGDSVKGRFAISRDNAKNTLYLQM
		NSLKPEDTAMYYCAAGPPPCITSQVQLQES
		GGGSVQAGGSLRLSCASSGYISSSYCMAWF
		RQAPGKEREGAAGVTMPAGGDYGYRYWGQG
		TQVTVSS

83	Anti-	QVQLQESGGALVQPGGSLRLSCAASGFTFS
	mouseGp130	YYAMKWVRQAPGKGLEWVSSISGGGGATYY
		ADSVKGRFTISRDNTNDTLYLQMNSLKTED
		TAVYYCAAQNLDYRGQGTQVTVSS

84	Anti-	QVQLQESGGGLVQPGGSLRLSCTASGFTFN
	mouseGp130	SAHLKWERQPPGKGLEWVSFITNGGASTGY
		ADSVKGRFTISRDDAKNTLYLQMNNLKTED
		TAVYYCATGGLRGQGTQVTVSS

85	Anti-	QVQLQESGGGLVQPGGSLRLSCAASGFTLS
	mouseGp130	TYWMYWVRQAPGKGPEWVSAVSRGGFNTYY
		ADSVKGRFTISRDNAKNTVYLQMNSLKPED
		TAVYYCMSSVSFYGWPPDRVPSPTGQGTQV
		TVSS

86	Anti-	QVQLQESGGGSVQPGGSLRLSCAASGFTFS
	mouseGp130	TYDMSWVRQAPGKGLEWVSTINYSGSSTYY
		VDSVLGRFTIARDNAKNTLYLQMNNLQTED
		TAVYYCASVKERRSNGHPIVFGDRGQGTQV
		TVSS

87	Anti-	QVQLQESGGGLVQPGGSLRLSCAASGFTFR
	mouseGp130	NYAMSWVRQAPGKGLEWVSAINSGGGSTYY
		ADSVKGRFTISRDNAKNTLYLQMNSLKPED
		TAMYYCAKHVTGDYDPSLRYEYNYWSQGTQ
		VTVSS

88	Anti-	QVQLQESGGGSVQAGGSLRLSCVISGFTYR
	mouseGp130	QTFMGWFRQVVGKEREGVAAISTGGGSTIY
		ADSVKGRFTISQDSSKDTVYLEMNGLKLED
		TGMYYCAASTVITSESINRNLYQYWGQGTQ
		VTVSS

89	Anti-	QVQLQESGGGSVQAGGFLRLSCAFSGYTGC
	mouseGp130	MGWFRQGPGQEREGVASINDGGSLTYADSV
		KGRFTISKDNAKKTLDLQMNTLKPEDTAMY
		YCAASLSYCLNPTLRVDGYNYWGQGTQVTV
		SS

90	Anti-	QVQLQESGGGLVQPGGSLRLSCAASGFTFS
	IL2Rbeta/anti-	LYDMSWVRQAPGKGLEWVSGINSGGYSTYY
	CD122 (mouse)	AASAKGRFTISRDNAKNTLYLQLSSVKTED
		TAMYYCAQRGLTSPYVIPNIRLOGTQVTVS
		S

91	Anti-	QVQLQESGGGLVQPGGSLRLSCAASEFTFS
	IL2Rbeta/anti-	NNWMHWVRQAPGKGFEWVSSIHSGMAITHY
	CD 122 (mouse)	RGSVKGRFTISSDIAKNIVSLQMNSLKAED
		TAVYYCVGEGNWGQGTQVTVSS

92	Anti-	QVQLQESGGGSVLAGGSLRLSCVASGYGYN
	IL2Rgamma/Anti-	YIGWFRQTPGKEREGVAVIYTGGGDTYYAD
	CD132	SVKGRFTASRDNAKSTLYLQMNSLEPEDTA
	(mouse)	MYYGVARYCVGSVYACLRGGHDEYAHWGQG
		TQVTVSS

93	Anti-	QVQLQESGGGSVQPGGSLRLSCAASGSTYA
	IL2Rgamma/Anti-	NYLMGWFRQAPGKEREGVAAIYSGGGSTYY
	CD132	ADSVKGRFTISQDNAKNTLYLQMNSLKPED
	(mouse)	TAMYYCAAASAVKGDKGDIVVVVTGTQRME
		YDYWGHGTQVTVSS

94	Anti-	QVQLQESGGGSVQAGASLRLSCSVSGFTFD
	IL2Rgamma/Anti-	ESVMSWLRQGPGNECDAVAIISSDDNTYYD
	CD132	DSVKGRFTISEDNAKNMVYLQMNSLKPEDT
	(mouse)	AVYYCAARRRRPVYDSDYELRPRPLCGDFG
		VWGQGTQVTVSS

95	Anti-	QVQLQESGGGSVQAGGSLRLSCIGSGLPFD
	IL2Rgamma/Anti-	EDDMGWYRQAPGNECELVSSISSDGTAYYA
	CD132	DSVKGRFTISRDNAKNTVLLQMNSLKPEDT
	(mouse)	AVYYCAAGVHRQFGGSSSCGDAFYGMDYWG
		KGTQVTVSS

96	Anti-	QVQLQESGGGSVQAGGSLRLSCVASGDVYG
	IL2Rgamma/Ant	RNSMAWFRQAPGKEREGVAVGYSVVTTTYY
	i-CD132	ADSVKGRFTISEDNDKNTVYLEMNSLKPED
	(mouse)	TAMYYCAADGNLWRGLRPSEYTYWGQGTQV
		TVSS

97	Anti-	QVQLQESGGGSVQAGGSLRLSCTASGFTFD
	IL2Rgamma/Anti-	DFDMGWYRQAPGNECELVSTISDDGSTYYA
	CD132	DSVKGRSSISRDNAKNTVYLQMNRLKPEDT
	(mouse)	GVYYCAAEGALGSKMNCGWVGNFGYWGQGT
		QVTVSS

98	Anti-	QVQLQESGGGSVQAGGSLRLSCATSGFPYS
	IL2Rgamma/Anti-	RYCMGWFRQAPGKEREGVAAIEPDGSTSYA
	CD132	DSVKGRFTISQDNAVNTLYLQMNNLKPEDT
	(mouse)	AMYYCAADERCFYLKDYDLRRPAQYRYWGQ
		GTQVTVSS

99	Anti-IL10Rbeta	QVQLQESGGGSVQAGGSLRLSCAASGYTYN
	(mouse)	RRFMGWFRQAPGKEREGLAIIYTPNSSTFY
		ADSVTGRFTISQDSARNTVYLQMNSLKPED
		TAMYYCAAARIASMTELSVRDMDYWGKGTQ
		VTVSS

100	Anti-IL10Rbeta	QVQLQESGGGSVQAGGSLRLSCTASRYIAL
	(mouse)	NACMAWIRQAPGSEREVVATIVTDGSRTYY
		ADSVKGRFTISQDNAKNTMYLQMNGLKPED
		TAMYYCAADRRCPVSRAPYEYELRYWGQGT
		QVTVSS

101	Anti-IL10Rbeta	QVQLQESGGGSVQAGGSLRLSCVASGDTYS
	(mouse)	RKYIAWVRQVPGKEREGVAVMYTPGSATYY
		TDTVMGRFTISQDNAKNTVYLQMNSLKPED
		TAMYFCAAKASGSMFNFRDYTYWGQGTQVT
		VSS

102	Anti-IL10Rbeta	QVQLQESGGGSVQAGGALRLSCTASGYTAS
	(mouse)	SICMGWFRQAPGKERERVAVITTAASGTYY
		ADSVNGRFSISQNNAKNTVYLQMNSLKPDD
		TAMYYCAATRRGGDCLDPLQTPAYNTWGQG
		TQVTVSS

103	Anti-IL10Rbeta	QVQLQESGGGSVQAGGSLRLSCATSGYASC
	(mouse)	SRAMRWYRQAPGKEREFVAYIDGVGSTGYA
		DSVKGRFTISQDNAKYTAYLQMNSLKPEDT
		AMYYCNRGCRADGSNSLDNYWGQGTQVTVS
		S

104	Anti-IL10Rbeta	QVQLQESGGGSVQAGGSLRLSCAASGYTYN
	(mouse)	GKCMAWFRQAPGKEREVVAGIYTGGSSTYY
		ADSVKGRFTISQDNAKNTVYLQMDSLKPED
		TAMYYCATSRSCSDLRRRSIAYWGQGTQVT
		VSS

105	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	(mouse)	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
		ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSS

106	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	(mouse)	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
		DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSS

107	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	(mouse)	GYDMMWYRQAPGKEREFVALITSDYSIRYE
		DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSS

108	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	(mouse)	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
		FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSS

109	Anti-IL12Rbeta1	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	(mouse)	DSEMGWYRQAPGHECELVASGSSDDDTYYV
		DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		S

110	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	(mouse)	SAFMAWFRQAPGKEREGVAAIYTRDGSPVY
		ADSLKGRFTISQDNAKNTLHLQMNSLKPED
		TAMYYCAAKIPEPGRISLLDSQTYDYWGHG
		TQVTVSS

111	Anti-IL12Rbeta1	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	(mouse)	GYDVRWYRRAPGKEREFVSGIDSDGSTSYA
		DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSS

112	Anti-IL12Rbeta2	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	(mouse)	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
		ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVS(303)

113	Anti-IL12Rbeta2	QVQLQESGGGSVQAGGSLRLSCAASGVTYG
	(mouse)	SYYMAAWFRQAPGKEREGVASIYGGSDSTY
		YADSVLGRFTISQDNGKNTLYLQMNSLKPD
		DTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSS

114	Anti-IL12Rbeta2	QVQLQESGGGSVQVGGSLRLSCAASGFTYS
	(mouse)	SSCLGWFRQAPGKEREGVATIYPAGGNIFY
		ADSVKGRFTISQDNAKNTVYLQMDSLKPED
		TAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSS

115	Anti-IL12Rbeta2	QVQLQESGGGSVQVGGSLRLSCAVSGKLYG
	(mouse)	GAWFRQAQGKGREGVAAIWIGTGTTFYADS
		VKGRFTISRDNAKNTVYLQMDGLKPEDTAL
		YYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSS

116	Anti-IL12Rbeta2	QVQLQESGGGSVQAGGSLRLSCAASGITYR
	(mouse)	GVWMGWFRQAPGKEREGVATIYTGSGHTYY
		ADSVKGRFTISQDNAKNTVYLQMNSLKPED
		TAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSS

117	Anti-IL12Rbeta2	QVQLQESGGGSVQDGGSLRLSCAASGDIYA
	(mouse)	RNCMGWFRQAPGKEREKIAVADTGGRSPYY
		ADSVKGRFTISRDNAKNTVDLQMNSLKPED
		TAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSS

118	Anti-il23R	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	mouse	SCTMGWYRQAPGKERELVSMLISDGSTFYA
		DSVKGRFTFSQEYAKNTVYLQMNSLKPEDT
		AMYYCGCATLGSRTVWGQGTQVTVSS

119	Anti-il23R	QVQLQESGGGSVQAGGSLTLSCTAPGFTFR
	mouse	LAAMRWVRQAPGKGLEWVSGIDSRGSTIYA
		DSVKGRFTISKDNAKNTLYLQLNSLKTEDT
		AMYYCAQGVYGDTYSGSQGTQVTVSS

120	Anti-il23R	QVQLQESGGGSVQAGGSLRLSCTASVNTYC
	mouse	EYNMSWYRQAPGKEREFVSGVDSDGSTRYS
		ESVKGRFTISQDNAKNTMYLQMNGLKPEDT
		AMYYCKTYVCTFCSGNSCYYEYKYYYEGQG
		TQVTVSS

121	Anti-il23R	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	mouse	NNCMGWFRQAPGKDRERIANIYTGGGRTTY
		ADSVKGRFTISQDSAKSTVYLQMNSLKPED
		TAMYYCAAGSCGSARSEYSYWGQGTQVTVS
		S

122	Anti-il23R	QVQLQESGGGSVQAGGSLRLSCAASGYTFC
	mouse	MAWFRQAPGKEREGVARFYTRDGYTYYSDS
		VKGRFTISQNNAKNTLYLQMNSLKSEDTAM
		YYCAADLARCSSNKNDFRYWGQGTQVTVSS

123	Anti-il23R	QVQLQESGGGSVQAGGSLRLSCAASGYTSG
	mouse	NYWMGWFRQAPGKEREGVATLWTGGASTFY
		GDSVKGRFTISRDNFKNTLYLQMNSLKVED
		TAMYYCAADPALRLGANILRPAEYKYWGQG
		TQVTVSS

124	Anti-il23R	QVQLQESGGGLVQPGGSLRLSCAASGFTFS
	mouse	RSAMTWVRQAPGKGLDWVSGIDSGGTTVYA
		DSVKGRFTISRDSAKNTLYLQMNSLKTEDT
		AVYYCAIGLPWGNTWRTRGQGTQVTVSS

125	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCAVSGDSTY
	(mouse)	SMGWFRQPPGKEREGVAAITKDITIHADSV
		KGRFTISKDNAKNTLYLQMNSLKPEDTAMY
		YCAAHRPYGPPLNPRWYTYWGQGTQVTVSS

126	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCTASGYTSS
	(mouse)	RYCMGWFRQTPGKKREGVAAIYTGGGTTFY
		HGSVKGRFTISQDNTTNTVYLQMHNLKPED
		TAMYYCAAGPVTRACDEYNYWGQGTQVTVS
		S

127	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCAASGYSIN
	(mouse)	RMGWFRQAPGKEREGVAAISIGGGQTYYAD
		SVKGRFTISQDNAKNTVDLQMNSLKPEDTA
		MYYCAAGLVYGEAWLDSRHYNKWGQGTQVT
		VSS

128	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCAGSGYSLS
	(mouse)	NYCMGWFRQAPGQGREGVASLRFVSGATFY
		ADSVKGRFTIAQDNAKNTLYLQMNSLKPED
		TAMYYCGIKSRGICGGRLVDVDFGNWGQGT
		QVTVSS

129	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCAASKNSNF
	(mouse)	MGWFRQAPGKEREGVAAMMTKNNNTYYADS
		VKGRFTISHDNAKNTVYLQMDSLKPEDTAV
		YYCAAVYRTRRLRVLEAANFDYWGQGTQVT
		VSS

130	Anti-il27R	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	(mouse)	SYCMAWFRQAPGKEREGVAAIDSDGSTSYA
		DSVKGRFTISKDNAKNTLYLQMNSLKPEDT
		AMYYCAAASGRCLGPGIRSLIWGQGTQVTV
		SS

131	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12Rβ2 V_HH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGYTYSNRHMGWFRQAPGKEREGVA
		AIYTGGGSTYYADSVKDRFTISQDNAKNTL
		YLQMNSLTPEDTAMYYCAADLTRWYSGGWR
		DPRGYKYWGQGTQVTVS
		(SEQ ID NO: 131)

132	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12Rβ2VHH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGVTYGSYYMAAWFRQAPGKEREGV
		ASIYGGSDSTYYADSVLGRFTISQDNGKNT
		LYLQMNSLKPDDTAMYYCAAAPPGKWFLKR
		LEGHNYSYWGQGTQVTVSS
		(SEQ ID NO: 132)

133	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12Rβ2 V_HH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQVGGSLR
		LSCAASGFTYSSSCLGWFRQAPGKEREGVA
		TIYPAGGNIFYADSVKGRFTISQDNAKNTV
		YLQMDSLKPEDTAMYYCAARGGQTWGSGGN
		RCSLWLPAYNYWGQGTQVTVSS
		(SEQ ID NO: 133)

134	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12Rβ2 V_HH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQVGGSLR
		LSCAVSGKLYGGAWFRQAQGKGREGVAAIW
		IGTGTTFYADSVKGRFTISRDNAKNTVYLQ
		MDGLKPEDTALYYCAADDRPGYRDPLAPVS
		YNHWGQGTQVTVSS
		(SEQ ID NO: 134)

135	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12R2 V_HH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGITYRGVWMGWFRQAPGKEREGVA
		TIYTGSGHTYYADSVKGRFTISQDNAKNTV
		YLQMNSLKPEDTAMYYCAARTVGGTFYTLA
		ADSFNTWGQGTQVTVSS
		(SEQ ID NO: 135)

136	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCTASGYTYS
	GGGS-	SAFMAWFRQAPGKEREGVAAIYTRDGGTVY
	IL12Rβ2 V_HH	ADSVKGRFTISQDNAKNTLYLQMNSLKAED
		TAMYYCAAKIPQPGRASLLDSQTYDYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQDGGSLR
		LSCAASGDIYARNCMGWFRQAPGKEREKIA
		VADTGGRSPYYADSVKGRFTISRDNAKNTV
		DLQMNSLKPEDTAVYYCAAGPLVPVVNTAA
		RCVYEYWGQGTQVTVSS
		(SEQ ID NO: 136)
137	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGYTYSNRHMGWFRQAPGKEREGVAA
		IYTGGGSTYYADSVKDRFTISQDNAKNTLY
		LQMNSLTPEDTAMYYCAADLTRWYSGGWRD
		PRGYKYWGQGTQVTVS
		(SEQ ID NO: 137)

138	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGVTYGSYYMAAWFRQAPGKEREGVA
		SIYGGSDSTYYADSVLGRFTISQDNGKNTL
		YLQMNSLKPDDTAMYYCAAAPPGKWFLKRL
		EGHNYSYWGQGTQVTVSS
		(SEQ ID NO: 138)

139	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQVGGSLRL
		SCAASGFTYSSSCLGWFRQAPGKEREGVAT
		IYPAGGNIFYADSVKGRFTISQDNAKNTVY
		LQMDSLKPEDTAMYYCAARGGQTWGSGGNR
		CSLWLPAYNYWGQGTQVTVSS
		(SEQ ID NO: 139)

140	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQVGGSLRL
		SCAVSGKLYGGAWFRQAQGKGREGVAAIWI
		GTGTTFYADSVKGRFTISRDNAKNTVYLQM
		DGLKPEDTALYYCAADDRPGYRDPLAPVSY
		NHWGQGTQVTVSS
		(SEQ ID NO: 140)

141	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGITYRGVWMGWFRQAPGKEREGVAT
		IYTGSGHTYYADSVKGRFTISQDNAKNTVY
		LQMNSLKPEDTAMYYCAARTVGGTFYTLAA
		DSFNTWGQGTQVTVSS
		(SEQ ID NO: 141)

142	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCAVSGYDYC
	GGGS-	GYDVRWYRQAPGKEREFVSGIDSDGSTSYA
	IL12Rβ2 V_HH	DSVKGRFTISQDNAENTSYLHMFSLKPEDT
		AMYYCKTESPAGESAWCRNFRGMDYWGKGT
		QVTVSSGGGSQVQLQESGGGSVQDGGSLRL
		SCAASGDIYARNCMGWFRQAPGKEREKIAV
		ADTGGRSPYYADSVKGRFTISRDNAKNTVD
		LQMNSLKPEDTAVYYCAAGPLVPVVNTAAR
		CVYEYWGQGTQVTVSS
		(SEQ ID NO: 142)

143	IL12Rβ1VHH-	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12R2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGYTYSNRHMGWFRQAPGKEREGVAA
		IYTGGGSTYYADSVKDRFTISQDNAKNTLY
		LQMNSLTPEDTAMYYCAADLTRWYSGGWRD
		PRGYKYWGQGTQVTVS
		(SEQ ID NO: 143)

144	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	-GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12Rβ2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGVTYGSYYMAAWFRQAPGKEREGVA
		SIYGGSDSTYYADSVLGRFTISQDNGKNTL
		YLQMNSLKPDDTAMYYCAAAPPGKWFLKRL
		EGHNYSYWGQGTQVTVSS
		(SEQ ID NO: 144)

145	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	-GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12Rβ2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQVGGSLRL
		SCAASGFTYSSSCLGWFRQAPGKEREGVAT
		IYPAGGNIFYADSVKGRFTISQDNAKNTVY
		LQMDSLKPEDTAMYYCAARGGQTWGSGGNR
		CSLWLPAYNYWGQGTQVTVSS
		(SEQ ID NO: 145)

146	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	-GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12R2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQVGGSLRL
		SCAVSGKLYGGAWFRQAQGKGREGVAAIWI
		GTGTTFYADSVKGRFTISRDNAKNT137VY
		LQMDGLKPEDTALYYCAADDRPGYRDPL
		APVSYNHWGQGTQVTVSS
		(SE138Q ID NO: 149)

147	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	-GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12Rβ2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASGITYRGVWMGWFRQAPGKEREGVAT
		IYTGSGHTYYADSVKGRFTISQDNAKNTVY
		LQMNSLKPEDTAMYYCAARTVGGTFYTLAA
		DSFNTWGQGTQVTVSS
		(SEQ ID NO: 147)

148	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCVASGYSYC
	-GGGS-	GYDMMWYRQAPGKEREFVALITSDYSIRYE
	IL12R2 V_HH	DSVEGRFSISRDNAKNTGYLLMSNLTPADT
		AIYYCKTSTAARESSWCRSRYRVASWGQGT
		QVTVSSGGGSQVQLQESGGGSVQDGGSLRL
		SCAASGDIYARNCMGWFRQAPGKEREKIAV
		ADTGGRSPYYADSVKGRFTISRDNAKNTVD
		LQMNSLKPEDTAVYYCAAGPLVPVVNTAAR
		CVYEYWGQGTQVTVSS
		(SEQ ID NO: 148)

149	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGYTYSNRHMGWFRQAPGKEREGVA
		AIYTGGGSTYYADSVKDRFTISQDNAKNTL
		YLQMNSLTPEDTAMYYCAADLTRWYSGGWR
		DPRGYKYWGQGTQVTVS
		(SEQ ID NO: 149)

150	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGVTYGSYYMAAWFRQAPGKEREGV
		ASIYGGSDSTYYADSVLGRFTISQDNGKNT
		LYLQMNSLKPDDTAMYYCAAAPPGKWFLKR
		LEGHNYSYWGQGTQVTVSS
		(SEQ ID NO: 150)

151	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQVGGSLR
		LSCAASGFTYSSSCLGWFRQAPGKEREGVA
		TIYPAGGNIFYADSVKGRFTISQDNAKNTV
		YLQMDSLKPEDTAMYYCAARGGQTWGSGGN
		RCSLWLPAYNYWGQGTQVTVSS
		(SEQ ID NO: 151)

152	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQVGGSLR
		LSCAVSGKLYGGAWFRQAQGKGREGVAAIW
		IGTGTTFYADSVKGRFTISRDNAKNTVYLQ
		MDGLKPEDTALYYCAADDRPGYRDPLAPVS
		YNHWGQGTQVTVSS
		(SEQ ID NO: 152)

153	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQAGGSLR
		LSCAASGITYRGVWMGWFRQAPGKEREGVA
		TIYTGSGHTYYADSVKGRFTISQDNAKNTV
		YLQMNSLKPEDTAMYYCAARTVGGTFYTLA
		ADSFNTWGQGTQVTVSS
		(SEQ ID NO: 153)

154	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASRYTYT
	-GGGS-	NNFMAWFRQAPGKEREGVAAIYTGDGYAYY
	IL12Rβ2 V_HH	FDSVKGRFTISQDNDKNMLYLQMNSLKPED
		TAMYYCAAMERRSGRRRMTENAEYKYWGQG
		TQVTVSSGGGSQVQLQESGGGSVQDGGSLR
		LSCAASGDIYARNCMGWFRQAPGKEREKIA
		VADTGGRSPYYADSVKGRFTISRDNAKNTV
		DLQMNSLKPEDTAVYYCAAGPLVPVVNTAA
		RCVYEYWGQGTQVTVSS
		(SEQ ID NO: 154)

155	IL12Rβ1 V_HH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12Rβ2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GYTYSNRHMGWFRQAPGKEREGVAAIYTGG
		GSTYYADSVKDRFTISQDNAKNTLYLQMNS
		LTPEDTAMYYCAADLTRWYSGGWRDPRGYK
		YWGQGTQVTVS
		(SEQ ID NO: 155)

156	IL12Rβ1 V_HH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12Rβ2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GVTYGSYYMAAWFRQAPGKEREGVASIYGG
		SDSTYYADSVLGRFTISQDNGKNTLYLQMN
		SLKPDDTAMYYCAAAPPGKWFLKRLEGHNY
		SYWGQGTQVTVSS
		(SEQ ID NO: 156)

157	IL12Rβ1 V_HH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12R2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQVGGSLRLSCAAS
		GFTYSSSCLGWFRQAPGKEREGVATIYPAG
		GNIFYADSVKGRFTISQDNAKNTVYLQMDS
		LKPEDTAMYYCAARGGQTWGSGGNRCSLWL
		PAYNYWGQGTQVTVSS
		(SEQ ID NO: 157)

158	IL12Rβ1VHH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12Rβ2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQVGGSLRLSCAVS
		GKLYGGAWFRQAQGKGREGVAAIWIGTGTT
		FYADSVKGRFTISRDNAKNTVYLQMDGLKP
		EDTALYYCAADDRPGYRDPLAPVSYNHWGQ
		GTQVTVSS
		(SEQ ID NO: 158)

159	IL12Rβ1 V_HH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12Rβ2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GITYRGVWMGWFRQAPGKEREGVATIYTGS
		GHTYYADSVKGRFTISQDNAKNTVYLQMNS
		LKPEDTAMYYCAARTVGGTFYTLAADSFNT
		WGQGTQVTVSS
		(SEQ ID NO: 159)

160	IL12Rβ1 V_HH	QVQLQESGGGSVQAGETLRLSCTVSGFTID
	-GGGS-	DSEMGWYRQAPGHECELVASGSSDDDTYYV
	IL12Rβ2 V_HH	DSVKGRFTISLDNAKNMVYLQMNSLKPEDT
		AVYYCATGPTYPPKDGDCAHWGQGTQVTVS
		SGGGSQVQLQESGGGSVQDGGSLRLSCAAS
		GDIYARNCMGWFRQAPGKEREKIAVADTGG
		RSPYYADSVKGRFTISRDNAKNTVDLQMNS
		LKPEDTAVYYCAAGPLVPVVNTAARCVYEY
		WGQGTQVTVSS
		(SEQ ID NO: 160)

161	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	-GGGS-	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
	IL12Rβ2VHH	ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVSGGGSQVQLQESGGGSVQAGGSLRL
		SCTASGYTYSSAFMAWFRQAPGKEREGVAA
		IYTRDGGTVYADSVKGRFTISQDNAKNTLY
		LQMNSLKAEDTAMYYCAAKIPQPGRASLLD
		SQTYDYWGQGTQVTVSS
		(SEQ ID NO: 161)

162	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	-GGGS-	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
	IL12Rβ2 V_HH	ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVSGGGSQVQLQESGGGSVQAGGSLRL
		SCAVSGYDYCGYDVRWYRQAPGKEREFVSG
		IDSDGSTSYADSVKGRFTISQDNAENTSYL
		HMFSLKPEDTAMYYCKTESPAGESAWCRNF
		RGMDYWGKGTQVTVSS
		(SEQ ID NO: 162)

163	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	-GGGS-	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
	IL12Rβ2 V_HH	ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVSGGGSQVQLQESGGGSVQAGGSLRL
		SCVASGYSYCGYDMMWYRQAPGKEREFVAL
		ITSDYSIRYEDSVEGRFSISRDNAKNTGYL
		LMSNLTPADTAIYYCKTSTAARESSWCRSR
		YRVASWGQGTQVTVSS
		(SEQ ID NO: 163)

164	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	-GGGS-	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
	IL12Rβ2 V_HH	ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVSGGGSQVQLQESGGGSVQAGGSLRL
		SCAASRYTYTNNFMAWFRQAPGKEREGVAA
		IYTGDGYAYYFDSVKGRFTISQDNDKNMLY
		LQMNSLKPEDTAMYYCAAMERRSGRRRMTE
		NAEYKYWGQGTQVTVSS
		(SEQ ID NO: 164)

165	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGYTYS
	-GGGS-	NRHMGWFRQAPGKEREGVAAIYTGGGSTYY
	IL12Rβ2 V_HH	ADSVKDRFTISQDNAKNTLYLQMNSLTPED
		TAMYYCAADLTRWYSGGWRDPRGYKYWGQG
		TQVTVSGGGSQVQLQESGGGSVQAGETLRL
		SCTVSGFTIDDSEMGWYRQAPGHECELVAS
		GSSDDDTYYVDSVKGRFTISLDNAKNMVYL
		QMNSLKPEDTAVYYCATGPTYPPKDGDCAH
		WGQGTQVTVSS
		(SEQ ID NO: 165)

166	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGVTYGSYYMAAWFRQ
	-GGGS-	APGKEREGVASIYGGSDSTYYADSVLGRFTISQDNGKNTL
	IL12Rβ2 V_HH	YLQMNSLKPDDTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTASGYT
		YSSAFMAWFRQAPGKEREGVAAIYTRDGGTVYADSVKGRF
		TISQDNAKNTLYLQMNSLKAEDTAMYYCAAKIPQPGRASL
		LDSQTYDYWGQGTQVTVSS
		(SEQ ID NO: 166)

167	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGVTYGSYYMAAWFRQ
	-GGGS-	APGKEREGVASIYGGSDSTYYADSVLGRFTISQDNGKNTL
	IL12Rβ2 V_HH	YLQMNSLKPDDTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYD
		YCGYDVRWYRQAPGKEREFVSGIDSDGSTSYADSVKGRFT
		ISQDNAENTSYLHMFSLKPEDTAMYYCKTESPAGESAWCR
		NFRGMDYWGKGTQVTVSS
		(SEQ ID NO: 167)

168	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGVTYGSYYMAAWFRQ
	-GGGS-	APGKEREGVASIYGGSDSTYYADSVLGRFTISQDNGKNTL
	IL12Rβ2 V_HH	YLQMNSLKPDDTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCVASGYS
		YCGYDMMWYRQAPGKEREFVALITSDYSIRYEDSVEGRFS
		ISRDNAKNTGYLLMSNLTPADTAIYYCKTSTAARESSWCR
		SRYRVASWGQGTQVTVSS
		(SEQ ID NO: 168)

169	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGVTYGSYYMAAWFRQ
	-GGGS-	APGKEREGVASIYGGSDSTYYADSVLGRFTISQDNGKNTL
	IL12Rβ2 V_HH	YLQMNSLKPDDTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYT
		YTNNFMAWFRQAPGKEREGVAAIYTGDGYAYYFDSVKGRF
		TISQDNDKNMLYLQMNSLKPEDTAMYYCAAMERRSGRRRM
		TENAEYKYWGQGTQVTVSS
		(SEQ ID NO: 169)

170	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGVTYGSYYMAAWFRQ
	-GGGS-	APGKEREGVASIYGGSDSTYYADSVLGRFTISQDNGKNTL
	IL12Rβ2 V_HH	YLQMNSLKPDDTAMYYCAAAPPGKWFLKRLEGHNYSYWGQ
		GTQVTVSSGGGSQVQLQESGGGSVQAGETLRLSCTVSGFT
		IDDSEMGWYRQAPGHECELVASGSSDDDTYYVDSVKGRFT
		ISLDNAKNMVYLQMNSLKPEDTAVYYCATGPTYPPKDGDC
		AHWGQGTQVTVSS
		(SEQ ID NO: 170)

171	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAASGFTYSSSCLGWFRQA
	-GGGS-	PGKEREGVATIYPAGGNIFYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMDSLKPEDTAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTAS
		GYTYSSAFMAWFRQAPGKEREGVAAIYTRDGGTVYADSVK
		GRFTISQDNAKNTLYLQMNSLKAEDTAMYYCAAKIPQPGR
		ASLLDSQTYDYWGQGTQVTVSS
		(SEQ ID NO: 171)

172	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAASGFTYSSSCLGWFRQA
	-GGGS-	PGKEREGVATIYPAGGNIFYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMDSLKPEDTAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVS
		GYDYCGYDVRWYRQAPGKEREFVSGIDSDGSTSYADSVKG
		RFTISQDNAENTSYLHMFSLKPEDTAMYYCKTESPAGESA
		WCRNFRGMDYWGKGTQVTVSS
		(SEQ ID NO: 172)

173	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAASGFTYSSSCLGWFRQA
	-GGGS-	PGKEREGVATIYPAGGNIFYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMDSLKPEDTAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCVAS
		GYSYCGYDMMWYRQAPGKEREFVALITSDYSIRYEDSVEG
		RFSISRDNAKNTGYLLMSNLTPADTAIYYCKTSTAARESS
		WCRSRYRVASWGQGTQVTVSS
		(SEQ ID NO: 173)

174	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAASGFTYSSSCLGWFRQA
	-GGGS-	PGKEREGVATIYPAGGNIFYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMDSLKPEDTAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		RYTYTNNFMAWFRQAPGKEREGVAAIYTGDGYAYYFDSVK
		GRFTISQDNDKNMLYLQMNSLKPEDTAMYYCAAMERRSGR
		RRMTENAEYKYWGQGTQVTVSS
		(SEQ ID NO: 174)

175	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAASGFTYSSSCLGWFRQA
	-GGGS-	PGKEREGVATIYPAGGNIFYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMDSLKPEDTAMYYCAARGGQTWGSGGNRCSLWLPAYNY
		WGQGTQVTVSSGGGSQVQLQESGGGSVQAGETLRLSCTVS
		GFTIDDSEMGWYRQAPGHECELVASGSSDDDTYYVDSVKG
		RFTISLDNAKNMVYLQMNSLKPEDTAVYYCATGPTYPPKD
		GDCAHWGQGTQVTVSS
		(SEQ ID NO: 175)

176	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAVSGKLYGGAWFRQAQGK
	-GGGS-	GREGVAAIWIGTGTTFYADSVKGRFTISRDNAKNTVYLQM
	IL12Rβ2 V_HH	DGLKPEDTALYYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSSGGGSQVQLQESGGGSVQAGGSLRLSCTASGYTYSSAF
		MAWFRQAPGKEREGVAAIYTRDGGTVYADSVKGRFTISQD
		NAKNTLYLQMNSLKAEDTAMYYCAAKIPQPGRASLLDSQT
		YDYWGQGTQVTVSS
		(SEQ ID NO: 176)

177	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAVSGKLYGGAWFRQAQGK
	-GGGS-	GREGVAAIWIGTGTTFYADSVKGRFTISRDNAKNTVYLQM
	IL12Rβ2 V_HH	DGLKPEDTALYYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYDYCGYD
		VRWYRQAPGKEREFVSGIDSDGSTSYADSVKGRFTISQDN
		AENTSYLHMFSLKPEDTAMYYCKTESPAGESAWCRNFRGM
		DYWGKGTQVTVSS
		(SEQ ID NO: 177)

178	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAVSGKLYGGAWFRQAQGK
	-GGGS-	GREGVAAIWIGTGTTFYADSVKGRFTISRDNAKNTVYLQM
	IL12Rβ2VHH	DGLKPEDTALYYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSSGGGSQVQLQESGGGSVQAGGSLRLSCVASGYSYCGYD
		MMWYRQAPGKEREFVALITSDYSIRYEDSVEGRFSISRDN
		AKNTGYLLMSNLTPADTAIYYCKTSTAARESSWCRSRYRV
		ASWGQGTQVTVSS
		(SEQ ID NO: 178)

179	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAVSGKLYGGAWFRQAQGK
	-GGGS-	GREGVAAIWIGTGTTFYADSVKGRFTISRDNAKNTVYLQM
	IL12Rβ2 V_HH	DGLKPEDTALYYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTYTNNF
		MAWFRQAPGKEREGVAAIYTGDGYAYYFDSVKGRFTISQD
		NDKNMLYLQMNSLKPEDTAMYYCAAMERRSGRRRMTENAE
		YKYWGQGTQVTVSS
		(SEQ ID NO: 179)

180	IL12Rβ1 V_HH	QVQLQESGGGSVQVGGSLRLSCAVSGKLYGGAWFRQAQGK
	-GGGS-	GREGVAAIWIGTGTTFYADSVKGRFTISRDNAKNTVYLQM
	IL12Rβ2 V_HH	DGLKPEDTALYYCAADDRPGYRDPLAPVSYNHWGQGTQVT
		VSSGGGSQVQLQESGGGSVQAGETLRLSCTVSGFTIDDSE
		MGWYRQAPGHECELVASGSSDDDTYYVDSVKGRFTISLDN
		AKNMVYLQMNSLKPEDTAVYYCATGPTYPPKDGDCAHWGQ
		GTQVTVSS
		(SEQ ID NO: 180)

181	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGITYRGVWMGWFRQA
	-GGGS-	PGKEREGVATIYTGSGHTYYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMNSLKPEDTAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTASGYTYS
		SAFMAWFRQAPGKEREGVAAIYTRDGGTVYADSVKGRFTI
		SQDNAKNTLYLQMNSLKAEDTAMYYCAAKIPQPGRASLLD
		SQTYDYWGQGTQVTVSS
		(SEQ ID NO: 181)

182	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGITYRGVWMGWFRQA
	-GGGS-	PGKEREGVATIYTGSGHTYYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMNSLKPEDTAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYDYC
		GYDVRWYRQAPGKEREFVSGIDSDGSTSYADSVKGRFTIS
		QDNAENTSYLHMFSLKPEDTAMYYCKTESPAGESAWCRNF
		RGMDYWGKGTQVTVSS
		(SEQ ID NO: 182)

183	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGITYRGVWMGWFRQA
	-GGGS-	PGKEREGVATIYTGSGHTYYADSVKGRFTISQDNAKNTVY
	IL12Rβ2VHH	LQMNSLKPEDTAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCVASGYSYC
		GYDMMWYRQAPGKEREFVALITSDYSIRYEDSVEGRFSIS
		RDNAKNTGYLLMSNLTPADTAIYYCKTSTAARESSWCRSR
		YRVASWGQGTQVTVSS
		(SEQ ID NO: 183)

184	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGITYRGVWMGWFRQA
	-GGGS-	PGKEREGVATIYTGSGHTYYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMNSLKPEDTAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTYT
		NNFMAWFRQAPGKEREGVAAIYTGDGYAYYFDSVKGRFTI
		SQDNDKNMLYLQMNSLKPEDTAMYYCAAMERRSGRRRMTE
		NAEYKYWGQGTQVTVSS
		(SEQ ID NO: 184)

185	IL12Rβ1 V_HH	QVQLQESGGGSVQAGGSLRLSCAASGITYRGVWMGWFRQA
	-GGGS-	PGKEREGVATIYTGSGHTYYADSVKGRFTISQDNAKNTVY
	IL12Rβ2 V_HH	LQMNSLKPEDTAMYYCAARTVGGTFYTLAADSFNTWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGETLRLSCTVSGFTID
		DSEMGWYRQAPGHECELVASGSSDDDTYYVDSVKGRFTIS
		LDNAKNMVYLQMNSLKPEDTAVYYCATGPTYPPKDGDCAH
		WGQGTQVTVSS
		(SEQ ID NO: 185)

186	IL12Rβ1 V_HH	QVQLQESGGGSVQDGGSLRLSCAASGDIYARNCMGWFRQA
	-GGGS-	PGKEREKIAVADTGGRSPYYADSVKGRFTISRDNAKNTVD
	IL12Rβ2 V_HH	LQMNSLKPEDTAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTASGYTYS
		SAFMAWFRQAPGKEREGVAAIYTRDGGTVYADSVKGRFTI
		SQDNAKNTLYLQMNSLKAEDTAMYYCAAKIPQPGRASLLD
		SQTYDYWGQGTQVTVSS
		(SEQ ID NO: 186)

187	IL12Rβ1 V_HH	QVQLQESGGGSVQDGGSLRLSCAASGDIYARNCMGWFRQA
	-GGGS-	PGKEREKIAVADTGGRSPYYADSVKGRFTISRDNAKNTVD
	IL12Rβ2 V_HH	LQMNSLKPEDTAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYDYC
		GYDVRWYRQAPGKEREFVSGIDSDGSTSYADSVKGRFTIS
		QDNAENTSYLHMFSLKPEDTAMYYCKTESPAGESAWCRNF
		RGMDYWGKGTQVTVSS
		(SEQ ID NO: 187)

188	IL12Rβ1 V_HH	QVQLQESGGGSVQDGGSLRLSCAASGDIYARNCMGWFRQA
	-GGGS-	PGKEREKIAVADTGGRSPYYADSVKGRFTISRDNAKNTVD
	IL12Rβ2 V_HH	LQMNSLKPEDTAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCVASGYSYC
		GYDMMWYRQAPGKEREFVALITSDYSIRYEDSVEGRFSIS
		RDNAKNTGYLLMSNLTPADTAIYYCKTSTAARESSWCRSR
		YRVASWGQGTQVTVSS
		(SEQ ID NO: 188)

189	IL12Rβ1 V_HH	QVQLQESGGGSVQDGGSLRLSCAASGDIYARNCMGWFRQA
	-GGGS-	PGKEREKIAVADTGGRSPYYADSVKGRFTISRDNAKNTVD
	IL12Rβ2 V_HH	LQMNSLKPEDTAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTYT
		NNFMAWFRQAPGKEREGVAAIYTGDGYAYYFDSVKGRFTI
		SQDNDKNMLYLQMNSLKPEDTAMYYCAAMERRSGRRRMTE
		NAEYKYWGQGTQVTVSS
		(SEQ ID NO: 189)

190	IL12Rβ1 V_HH	QVQLQESGGGSVQDGGSLRLSCAASGDIYARNCMGWFRQA
	-GGGS-	PGKEREKIAVADTGGRSPYYADSVKGRFTISRDNAKNTVD
	IL12Rβ2 V_HH	LQMNSLKPEDTAVYYCAAGPLVPVVNTAARCVYEYWGQGT
		QVTVSSGGGSQVQLQESGGGSVQAGETLRLSCTVSGFTID
		DSEMGWYRQAPGHECELVASGSSDDDTYYVDSVKGRFTIS
		LDNAKNMVYLQMNSLKPEDTAVYYCATGPTYPPKDGDCAH
		WGQGTQVTVSS
		(SEQ ID NO: 190)

191	linker	GSGSGSGS

192	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSS
	ASH6	GCMGWFRQAPGKEREAVAAINSDGSTSYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGYPRWSVA
		EFGYWGQGTQVTVSSASHHHHHH

193	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSS
	ASH6	YCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGYCDGGPN
		KYWGQGTQVTVSSASHHHHHH

194	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTYNS
	ASH6	YCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAAMTTNPL
		GQGTQVTVSSASHHHHHH

195	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSRYTASV
	ASH6	NYMGWFRQAPGKEREGVATIFTGAGTTYYANSVKGRFTIS
		RDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLLYRPAYE
		YTYRGQGTQVTVSSASHHHHHH

196	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAASGYTHSS
	ASH6	YCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSNYFLPPG
		AVRYWGQGTQVTVSSASHHHHHH

197	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSYSS
	ASH6	YCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSGAVGRNP
		PYWGQGTQVTVSSASHHHHHH

198	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMAWFRQS
	VHH-	PGKEREPVAVIYTASGATFYPDSVKGRFTISQDNAKMTVY
	GGGS-	LQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYWGQGTQ
	IL10RβVHH-	VTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAASGYTYLR
	ASH6	GCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVKGRFTIS
		RDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGWRSGLDY
		WGQGTQVTVSSASHHHHHH

199	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	VHH-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	GGGS-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	IL10RβVHH-	KGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGY
	ASH6	TYSSGCMGWFRQAPGKEREAVAAINSDGSTSYADSVKGRF
		TISKDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGYPR
		WSVAEFGYWGQGTQVTVSSASHHHHHH

200	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	VHH-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	GGGS-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	IL10RβVHH-	KGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGY
	ASH6	TYSSYCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKGRF
		TISKDNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGYCD
		GGPNKYWGQGTQVTVSSASHHHHHH

201	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	VHH-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	GGGS-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	IL10Rα	KGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRY
	VHH-	TYNSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRF
	ASH6	TISKDNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAAMT
		TNPLGQGTQVTVSSASHHHHHH

202	IL10Rα	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	VHH-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	GGGS-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	IL10RβVHH-	KGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSRY
	ASH6	TASVNYMGWFRQAPGKEREGVATIFTGAGTTYYANSVKGR
		FTISRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLLYR
		PAYEYTYRGQGTQVTVSSASHHHHHH

203	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	GGGS-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	ASH6	KGTQVTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAASGY
		THSSYCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKGRF
		TISKDNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSNYF
		LPPGAVRYWGQGTQVTVSSASHHHHHH

204	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	GGGS-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	ASH6	KGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGY
		SYSSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRF
		TISKDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSGAV
		GRNPPYWGQGTQVTVSSASHHHHHH

205	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMGWFRQA
	GGGS-	PGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAGMDYWG
	ASH6	KGTQVTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAASGY
		TYLRGCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVKGR
		FTISRDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGWRS
		GLDYWGQGTQVTVSSASHHHHHH

206	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GYTYSSGCMGWFRQAPGKEREAVAAINSDGSTSYADSVKG
		RFTISKDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGY
		PRWSVAEFGYWGQGTQVTVSSASHHHHHH

207	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GYTYSSYCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKG
		RFTISKDNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGY
		CDGGPNKYWGQGTQVTVSSASHHHHHH

208	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		RYTYNSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKG
		RFTISKDNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAA
		MTTNPLGQGTQVTVSSASHHHHHH

209	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVS
		RYTASVNYMGWFRQAPGKEREGVATIFTGAGTTYYANSVK
		GRFTISRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLL
		YRPAYEYTYRGQGTQVTVSSASHHHHHH

210	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAAS
		GYTHSSYCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKG
		RFTISKDNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSN
		YFLPPGAVRYWGQGTQVTVSSASHHHHHH

211	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAAS
		GYSYSSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKG
		RFTISKDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSG
		AVGRNPPYWGQGTQVTVSSASHHHHHH

212	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMGWFRQA
	GGGS-	PGKEREGVAQINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYTYEYNY
	ASH6	WGQGTQVTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAAS
		GYTYLRGCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVK
		GRFTISRDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGW
		RSGLDYWGQGTQVTVSSASHHHHHH

213	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSC
		AASGYTYSSGCMGWFRQAPGKEREAVAAINSDGSTSYADS
		VKGRFTISKDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCS
		GGYPRWSVAEFGYWGQGTQVTVSSASHHHHHH

214	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSC
		AASGYTYSSYCMGWFRQAPGKEREGVAHIDSDGSTSYADS
		VKGRFTISKDNAKNTLYLQMNSLKPEDTAMYYCAADPIPG
		PGYCDGGPNKYWGQGTQVTVSSASHHHHHH

215	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSC
		AASRYTYNSYCMGWFRQAPGKEREGVATIDSDGMTRYADS
		VKGRFTISKDNAKNTLYLQMNSLKPEDTAMYYCAADADCT
		IAAMTTNPLGQGTQVTVSSASHHHHHH

216	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSC
		TVSRYTASVNYMGWFRQAPGKEREGVATIFTGAGTTYYAN
		SVKGRFTISRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRG
		GLLYRPAYEYTYRGQGTQVTVSSASHHHHHH

217	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVEAGGSLRLSC
		AASGYTHSSYCMGWFRQAPGKEREGVAAIDVDGSTTYADS
		VKGRFTISKDNAKNTLYLQMNSLKPEDTGMYYCAAEFADC
		SSNYFLPPGAVRYWGQGTQVTVSSASHHHHHH

218	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSC
		AASGYSYSSYCMGWFRQAPGKEREGVATIDSDGMTRYADS
		VKGRFTISKDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDC
		DSGAVGRNPPYWGQGTQVTVSSASHHHHHH

219	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMGWFRQA
	GGGS-	PGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAKNTLYL
	IL10RβVHH-	RMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIKVSKAD
	ASH6	FRYWGQGTQVTVSSGGGSQVQLQESGGGSVQTGGSLRLSC
		AASGYTYLRGCMGWFRQAPGKEREGVAVMDVVGDRRSYID
		SVKGRFTISRDNAANSVYLQMDNLKPEDTAMYYCTAGPNC
		VGWRSGLDYWGQGTQVTVSSASHHHHHH

220	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTY
		SSGCMGWFRQAPGKEREAVAAINSDGSTSYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGYPRWS
		VAEFGYWGQGTQVTVSSASHHHHHH

221	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTY
		SSYCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGYCDGG
		PNKYWGQGTQVTVSSASHHHHHH

222	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTY
		NSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAAMTTN
		PLGQGTQVTVSSASHHHHHH

223	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSRYTA
		SVNYMGWFRQAPGKEREGVATIFTGAGTTYYANSVKGRFT
		ISRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLLYRPA
		YEYTYRGQGTQVTVSSASHHHHHH

224	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAASGYTH
		SSYCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSNYFLP
		PGAVRYWGQGTQVTVSSASHHHHHH

225	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS-	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSY
		SSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSGAVGR
		NPPYWGQGTQVTVSSASHHHHHH

226	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMGWFRQA
	GGGS	PGKEREGVATIYTGGGNTYYADSVKGRFTISQDNAKNTVY
	IL10RβVHH-	LQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFDYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAASGYTY
		LRGCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVKGRFT
		ISRDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGWRSGL
		DYWGQGTQVTVSSASHHHHHH

227	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYS
		SGCMGWFRQAPGKEREAVAAINSDGSTSYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGYPRWSV
		AEFGYWGQGTQVTVSSASHHHHHH

228	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYS
		SYCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGYCDGGP
		NKYWGQGTQVTVSSASHHHHHH

229	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTYN
		SYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAAMTTNP
		LGQGTQVTVSSASHHHHHH

230	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSRYTAS
		VNYMGWFRQAPGKEREGVATIFTGAGTTYYANSVKGRFTI
		SRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLLYRPAY
		EYTYRGQGTQVTVSSASHHHHHH

231	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAASGYTHS
		SYCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSNYFLPP
		GAVRYWGQGTQVTVSSASHHHHHH

232	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSYS
		SYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSGAVGRN
		PPYWGQGTQVTVSSASHHHHHH

233	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMGWFRQV
	GGGS-	PGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGKNTLYL
	IL10RβVHH-	QMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDYWGKGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAASGYTYL
		RGCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVKGRFTI
		SRDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGWRSGLD
		YWGQGTQVTVSSASHHHHHH

234	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTY
		SSGCMGWFRQAPGKEREAVAAINSDGSTSYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAAEPYCSGGYPRWS
		VAEFGYWGQGTQVTVSSASHHHHHH

235	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTY
		SSYCMGWFRQAPGKEREGVAHIDSDGSTSYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAADPIPGPGYCDGG
		PNKYWGQGTQVTVSSASHHHHHH

236	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYTY
		NSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAADADCTIAAMTTN
		PLGQGTQVTVSSASHHHHHH

237	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSRYTA
		SVNYMGWFRQAPGKEREGVATIFTGAGTTYYANSVKGRFT
		ISRDNAKNTAYLQMNSLKPEDTAIYYCAVDFRGGLLYRPA
		YEYTYRGQGTQVTVSSASHHHHHH

238	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVEAGGSLRLSCAASGYTH
		SSYCMGWFRQAPGKEREGVAAIDVDGSTTYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTGMYYCAAEFADCSSNYFLP
		PGAVRYWGQGTQVTVSSASHHHHHH

239	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSY
		SSYCMGWFRQAPGKEREGVATIDSDGMTRYADSVKGRFTI
		SKDNAKNTLYLQMNSLKPEDTAMYYCAAPLYDCDSGAVGR
		NPPYWGQGTQVTVSSASHHHHHH

240	IL10Rα V_HH-	QVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMTWYRQA
	GGGS-	PGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAKNTVYL
	IL10RβVHH-	QMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRANYWGQG
	ASH6	TQVTVSSGGGSQVQLQESGGGSVQTGGSLRLSCAASGYTY
		LRGCMGWFRQAPGKEREGVAVMDVVGDRRSYIDSVKGRFT
		ISRDNAANSVYLQMDNLKPEDTAMYYCTAGPNCVGWRSGL
		DYWGQGTQVTVSSASHHHHHH

241	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYS
		IDYMAWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTI
		SQDNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQ
		SFTYWGQGTQVTVSSASHHHHHH

242	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYS
		SYCMGWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGF
		LLSAGMDYWGKGTQVTVSSASHHHHHH

243	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYS
		MYCMGWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERL
		CGPYTYEYNYWGQGTQVTVSSASHHHHHH

244	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYS
		TYCMGWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTIS
		KDNAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFL
		GPEIKVSKADFRYWGQGTQVTVSSASHHHHHH

245	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYS
		SNCMGWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTI
		SQDNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCP
		TPTFDYWGQGTQVTVSSASHHHHHH

246	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYS
		SYCMGWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTIS
		KDNGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLY
		LGMDYWGKGTQVTVSSASHHHHHH

247	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSGCMGWFRQA
	GGGS-	PGKEREAVAAINSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAEPYCSGGYPRWSVAEFGYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNC
		SYDMTWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFIS
		QDNAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWY
		SVRANYWGQGTQVTVSSASHHHHHH

248	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYSID
		YMAWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTISQ
		DNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSF
		TYWGQGTQVTVSSASHHHHHH

249	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYSSY
		CMGWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTISKD
		NAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGFLL
		SAGMDYWGKGTQVTVSSASHHHHHH

250	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSMY
		CMGWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTISKD
		NAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERLCG
		PYTYEYNYWGQGTQVTVSSASHHHHHH

251	IL10RVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYSTY
		CMGWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTISKD
		NAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGP
		EIKVSKADFRYWGQGTQVTVSSASHHHHHH

252	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYSSN
		CMGWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTISQ
		DNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTP
		TFDYWGQGTQVTVSSASHHHHHH

253	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYSSY
		CMGWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTISKD
		NGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLYLG
		MDYWGKGTQVTVSSASHHHHHH

254	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYTYSSYCMGWFRQA
	GGGS-	PGKEREGVAHIDSDGSTSYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADPIPGPGYCDGGPNKYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNCSY
		DMTWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFISQD
		NAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSV
		RANYWGQGTQVTVSSASHHHHHH

255	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYMA
		WFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTISQDNA
		KMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTYW
		GQGTQVTVSSASHHHHHH

256	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCMG
		WFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTISKDNAK
		NTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSAG
		MDYWGKGTQVTVSSASHHHHHH

257	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCMG
		WFRQAPGKEREGVAQINSDGSTSYADSVKGRFTISKDNAK
		NTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPYT
		YEYNYWGQGTQVTVSSASHHHHHH

258	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCMG
		WFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTISKDNAK
		NTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEIK
		VSKADFRYWGQGTQVTVSSASHHHHHH

259	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCMG
		WFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTISQDNA
		KNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTFD
		YWGQGTQVTVSSASHHHHHH

260	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCMG
		WFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTISKDNGK
		NTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMDY
		WGKGTQVTVSSASHHHHHH

261	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASRYTYNSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAADADCTIAAMTTNPLGQGTQVTVS
	ASH6	SGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDMT
		WYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFISQDNAK
		NTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRAN
		YWGQGTQVTVSSASHHHHHH

262	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYSI
		DYMAWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTIS
		QDNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQS
		FTYWGQGTQVTVSSASHHHHHH

263	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYSS
		YCMGWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGFL
		LSAGMDYWGKGTQVTVSSASHHHHHH

264	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSM
		YCMGWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTISK
		DNAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERLC
		GPYTYEYNYWGQGTQVTVSSASHHHHHH

265	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYST
		YCMGWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTISK
		DNAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFLG
		PEIKVSKADFRYWGQGTQVTVSSASHHHHHH

266	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYSS
		NCMGWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTIS
		QDNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCPT
		PTFDYWGQGTQVTVSSASHHHHHH

267	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYSS
		YCMGWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTISK
		DNGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLYL
		GMDYWGKGTQVTVSSASHHHHHH

268	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCTVSRYTASVNYMGWFRQA
	GGGS-	PGKEREGVATIFTGAGTTYYANSVKGRFTISRDNAKNTAY
	IL10Rα V_HH-	LQMNSLKPEDTAIYYCAVDFRGGLLYRPAYEYTYRGQGTQ
	ASH6	VTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNCS
		YDMTWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFISQ
		DNAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWYS
		VRANYWGQGTQVTVSSASHHHHHH

269	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYS
		IDYMAWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTI
		SQDNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQ
		SFTYWGQGTQVTVSSASHHHHHH

270	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYS
		SYCMGWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGF
		LLSAGMDYWGKGTQVTVSSASHHHHHH

271	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYS
		MYCMGWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTIS
		KDNAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERL
		CGPYTYEYNYWGQGTQVTVSSASHHHHHH

272	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYS
		TYCMGWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTIS
		KDNAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFL
		GPEIKVSKADFRYWGQGTQVTVSSASHHHHHH

273	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYS
		SNCMGWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTI
		SQDNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCP
		TPTFDYWGQGTQVTVSSASHHHHHH

274	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYS
		SYCMGWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTIS
		KDNGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLY
		LGMDYWGKGTQVTVSSASHHHHHH

275	IL10RβVHH-	QVQLQESGGGSVEAGGSLRLSCAASGYTHSSYCMGWFRQA
	GGGS-	PGKEREGVAAIDVDGSTTYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTGMYYCAAEFADCSSNYFLPPGAVRYWGQGT
	ASH6	QVTVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNC
		SYDMTWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFIS
		QDNAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWY
		SVRANYWGQGTQVTVSSASHHHHHH

276	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYSID
		YMAWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTISQ
		DNAKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSF
		TYWGQGTQVTVSSASHHHHHH

277	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYSSY
		CMGWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTISKD
		NAKNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGFLL
		SAGMDYWGKGTQVTVSSASHHHHHH

278	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSMY
		CMGWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTISKD
		NAKNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERLCG
		PYTYEYNYWGQGTQVTVSSASHHHHHH

279	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYSTY
		CMGWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTISKD
		NAKNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGP
		EIKVSKADFRYWGQGTQVTVSSASHHHHHH

280	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYSSN
		CMGWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTISQ
		DNAKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTP
		TFDYWGQGTQVTVSSASHHHHHH

281	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYSSY
		CMGWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTISKD
		NGKNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLYLG
		MDYWGKGTQVTVSSASHHHHHH

282	IL10RβVHH-	QVQLQESGGGSVQAGGSLRLSCAASGYSYSSYCMGWFRQA
	GGGS-	PGKEREGVATIDSDGMTRYADSVKGRFTISKDNAKNTLYL
	IL10Rα V_HH-	QMNSLKPEDTAMYYCAAPLYDCDSGAVGRNPPYWGQGTQV
	ASH6	TVSSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNCSY
		DMTWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFISQD
		NAKNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSV
		RANYWGQGTQVTVSSASHHHHHH

283	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCAASRYLYSIDYM
		AWFRQSPGKEREPVAVIYTASGATFYPDSVKGRFTISQDN
		AKMTVYLQMNSLKSEDTAMYYCAAVRKTDSYLFDAQSFTY
		WGQGTQVTVSSASHHHHHH

284	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCAASRFTYSSYCM
		GWFRQAPGKEREGVASIDSDGSTSYTDSVKGRFTISKDNA
		KNTLYLQMNSLKPEDTAMYYCALDLMSTVVPGFCGFLLSA
		GMDYWGKGTQVTVSSASHHHHHH

285	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYTYSMYCM
		GWFRQAPGKEREGVAQINSDGSTSYADSVKGRFTISKDNA
		KNTLYLQMNSLKPEDTAMYYCAADSRVYGGSWYERLCGPY
		TYEYNYWGQGTQVTVSSASHHHHHH

286	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCAVSGYAYSTYCM
		GWFRQAPGKEREGVAAIDSGGSTSYADSVKGRFTISKDNA
		KNTLYLRMNSLKPEDTAMYYCAAVPPPPDGGSCLFLGPEI
		KVSKADFRYWGQGTQVTVSSASHHHHHH

287	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCTVSGYTYSSNCM
		GWFRQAPGKEREGVATIYTGGGNTYYADSVKGRFTISQDN
		AKNTVYLQMNNLKPEDTAMYYCAAEPLSRVYGGSCPTPTF
		DYWGQGTQVTVSSASHHHHHH

288	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCGASGYTYSSYCM
		GWFRQVPGKEREGVAVIDSDGSTSYADSVKGRFTISKDNG
		KNTLYLQMNSLKPEDTAMYYCAADLGHYRPPCGVLYLGMD
		YWGKGTQVTVSSASHHHHHH

289	IL10RβVHH-	QVQLQESGGGSVQTGGSLRLSCAASGYTYLRGCMGWFRQA
	GGGS-	PGKEREGVAVMDVVGDRRSYIDSVKGRFTISRDNAANSVY
	IL10Rα V_HH-	LQMDNLKPEDTAMYYCTAGPNCVGWRSGLDYWGQGTQVTV
	ASH6	SSGGGSQVQLQESGGGSVQAGGSLRLSCAASGYSNCSYDM
		TWYRQAPGKEREFVSAIHSDGSTRYADSVKGRFFISQDNA
		KNTVYLQMNSLKPEDTAMYYCKTDPLHCRAHGGSWYSVRA
		NYWGQGTQVTVSSASHHHHHH

290	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	192	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGAGCGGCGGAGGAAGCGTGCAAGCTGGAGGCTCTCT
		GAGGCTGAGCTGTGCTGCCAGCGGCTACACTTATAGCAGC
		GGCTGTATGGGCTGGTTCAGACAAGCCCCCGGCAAGGAAA
		GGGAAGCCGTGGCCGCCATCAATTCCGATGGCAGCACAAG
		CTACGCCGACAGCGTGAAGGGAAGGTTCACAATCAGCAAG
		GACAACGCCAAGAACACACTCTATCTGCAGATGAACTCTC
		TGAAGCCAGAGGACACAGCCATGTACTACTGCGCCGCTGA
		GCCTTACTGTAGCGGCGGCTACCCAAGATGGAGCGTCGCT
		GAGTTCGGCTACTGGGGCCAAGGCACACAAGTGACTGTCT
		CGTCTGCTAGCCACCATCACCATCACCAC

291	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	193	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGAGCGGAGGAGGCAGCGTCCAAGCCGGAGGCTCTCT
		GAGGCTGAGCTGTGCTGCCAGCGGCTACACTTACAGCAGC
		TACTGCATGGGCTGGTTCAGACAAGCCCCCGGCAAGGAGA
		GAGAGGGCGTGGCTCACATCGACAGCGACGGCTCCACAAG
		CTACGCCGATAGCGTGAAGGGAAGGTTCACAATCTCCAAG
		GACAACGCCAAGAACACTCTGTACCTCCAGATGAACTCTC
		TGAAGCCAGAGGACACTGCCATGTACTACTGTGCCGCCGA
		TCCAATTCCCGGCCCCGGCTACTGCGATGGCGGCCCTAAC
		AAGTACTGGGGCCAAGGCACACAAGTGACTGTCTCGTCTG
		CTAGCCACCATCACCATCACCAC

292	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	194	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGTCCGGAGGAGGAAGCGTGCAAGCCGGCGGATCTCT
		GAGACTGAGCTGTGCCGCCTCTAGGTACACTTACAACAGC
		TACTGCATGGGCTGGTTCAGACAAGCCCCCGGCAAGGAAA
		GAGAGGGCGTGGCCACTATCGATAGCGACGGCATGACTAG
		GTACGCTGATAGCGTCAAGGGAAGGTTCACAATCTCCAAG
		GACAATGCTAAGAACACTCTGTACCTCCAGATGAACTCTC
		TGAAGCCAGAGGACACAGCCATGTACTACTGCGCTGCCGA
		TGCCGACTGCACTATCGCCGCCATGACTACTAATCCTCTG
		GGCCAAGGCACACAAGTGACTGTCTCGTCTGCTAGCCACC
		ATCACCATCACCAC

293	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	195	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGTCCGGCGGAGGCAGCGTCCAAGCCGGAGGATCTCT
		GAGGCTGAGCTGTACAGTGAGCAGATACACTGCCAGCGTG
		AACTACATGGGCTGGTTCAGACAAGCCCCCGGCAAAGAGA
		GAGAGGGCGTGGCCACAATCTTCACTGGCGCCGGCACAAC
		ATACTACGCCAACTCCGTCAAGGGAAGGTTCACAATCTCT
		AGGGACAACGCCAAGAACACTGCCTATCTGCAGATGAACT
		CCCTCAAGCCAGAGGACACTGCCATCTACTACTGCGCCGT
		GGATTTCAGAGGCGGACTGCTGTATAGGCCAGCCTACGAG
		TACACTTATAGGGGCCAAGGCACACAAGTGACAGTCTCGT
		CTGCTAGCCACCATCACCATCACCAC

294	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	196	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGAGCGGAGGAGGCAGCGTCGAAGCTGGAGGATCTCT
		GAGGCTGAGCTGTGCTGCCAGCGGCTACACTCACAGCAGC
		TACTGTATGGGCTGGTTCAGACAAGCCCCCGGCAAGGAGA
		GGGAAGGCGTGGCTGCCATCGACGTGGATGGCAGCACTAC
		TTACGCCGACAGCGTGAAGGGAAGGTTCACTATCAGCAAG
		GACAACGCCAAGAACACACTCTATCTGCAGATGAACAGCC
		TCAAGCCAGAGGACACTGGCATGTACTACTGCGCCGCCGA
		GTTCGCCGATTGCAGCAGCAACTACTTTCTGCCTCCCGGC
		GCCGTCAGATATTGGGGCCAAGGCACTCAAGTGACAGTCT
		CGTCTGCTAGCCACCATCACCATCACCAC

295	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	197	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGAGCGGAGGAGGAAGCGTCCAAGCCGGAGGATCTCT
		GAGACTGAGCTGCGCCGCTAGTGGCTACTCCTACAGCAGC
		TACTGCATGGGCTGGTTTAGGCAAGCCCCCGGCAAGGAGA
		GAGAAGGCGTGGCCACTATCGACAGCGACGGCATGACAAG
		GTACGCCGACAGCGTGAAGGGAAGGTTCACAATCAGCAAG
		GACAACGCCAAGAACACACTGTATCTGCAGATGAACTCTC
		TGAAGCCAGAGGACACTGCCATGTACTACTGTGCCGCTCC
		TCTGTACGACTGTGATAGCGGCGCTGTGGGCAGAAATCCA
		CCTTATTGGGGCCAAGGCACTCAAGTGACAGTCTCGTCTG
		CTAGCCACCATCACCATCACCAC

296	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGACTGAGCTGTGCCGCCTCTAGGTA
	Encoding	TCTGTACAGCATCGACTACATGGCTTGGTTCAGACAGAGC
	SEQ ID NO:	CCCGGCAAGGAGAGGGAGCCAGTGGCTGTCATCTACACTG
	198	CCTCCGGCGCCACATTCTATCCAGATAGCGTGAAGGGAAG
		GTTCACTATCAGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGACACTGCCATGT
		ACTACTGTGCCGCCGTGAGGAAGACAGATAGCTACCTCTT
		CGACGCCCAGAGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAAGTGCAGCTGC
		AAGAGAGCGGAGGCGGCAGCGTGCAGACTGGAGGCTCTCT
		GAGACTGAGCTGTGCTGCCAGCGGCTACACTTATCTGAGG
		GGCTGTATGGGCTGGTTTAGGCAAGCCCCCGGCAAGGAGA
		GAGAGGGCGTGGCCGTCATGGATGTGGTGGGCGATAGGAG
		AAGCTACATCGACAGCGTGAAGGGAAGGTTCACAATCTCT
		AGGGACAATGCCGCCAACAGCGTCTATCTGCAGATGGACA
		ATCTGAAGCCAGAGGACACAGCCATGTACTACTGCACTGC
		CGGCCCTAACTGTGTGGGCTGGAGAAGCGGACTGGATTAC
		TGGGGCCAAGGCACACAAGTGACAGTCTCGTCTGCTAGCC
		ACCATCACCATCACCAC

297	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGGCTGAGCTGTGCCGCCTCTAGGTT
	Encoding	CACATACAGCAGCTACTGCATGGGCTGGTTCAGACAAGCC
	SEQ ID NO:	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGCATCGATAGCG
	199	ATGGCTCCACTAGCTACACTGACAGCGTGAAGGGAAGGTT
		CACTATCAGCAAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACAGCCATGTACT
		ACTGTGCCCTCGATCTGATGAGCACAGTGGTGCCCGGCTT
		CTGTGGCTTTCTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGCGGAGGATCCC
		AAGTGCAGCTGCAAGAGAGCGGCGGAGGAAGCGTGCAAGC
		TGGAGGCTCTCTGAGGCTGAGCTGTGCTGCCAGCGGCTAC
		ACTTATAGCAGCGGCTGTATGGGCTGGTTCAGACAAGCCC
		CCGGCAAGGAAAGGGAAGCCGTGGCCGCCATCAATTCCGA
		TGGCAGCACAAGCTACGCCGACAGCGTGAAGGGAAGGTTC
		ACAATCAGCAAGGACAACGCCAAGAACACACTCTATCTGC
		AGATGAACTCTCTGAAGCCAGAGGACACAGCCATGTACTA
		CTGCGCCGCTGAGCCTTACTGTAGCGGCGGCTACCCAAGA
		TGGAGCGTCGCTGAGTTCGGCTACTGGGGCCAAGGCACAC
		AAGTGACTGTCTCGTCTGCTAGCCACCATCACCATCACCA
		C

298	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGGCTGAGCTGTGCCGCCTCTAGGTT
	Encoding	CACATACAGCAGCTACTGCATGGGCTGGTTCAGACAAGCC
	SEQ ID NO:	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGCATCGATAGCG
	200	ATGGCTCCACTAGCTACACTGACAGCGTGAAGGGAAGGTT
		CACTATCAGCAAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACAGCCATGTACT
		ACTGTGCCCTCGATCTGATGAGCACAGTGGTGCCCGGCTT
		CTGTGGCTTTCTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGCGGAGGATCCC
		AAGTGCAGCTGCAAGAGAGCGGAGGAGGCAGCGTCCAAGC
		CGGAGGCTCTCTGAGGCTGAGCTGTGCTGCCAGCGGCTAC
		ACTTACAGCAGCTACTGCATGGGCTGGTTCAGACAAGCCC
		CCGGCAAGGAGAGAGAGGGCGTGGCTCACATCGACAGCGA
		CGGCTCCACAAGCTACGCCGATAGCGTGAAGGGAAGGTTC
		ACAATCTCCAAGGACAACGCCAAGAACACTCTGTACCTCC
		AGATGAACTCTCTGAAGCCAGAGGACACTGCCATGTACTA
		CTGTGCCGCCGATCCAATTCCCGGCCCCGGCTACTGCGAT
		GGCGGCCCTAACAAGTACTGGGGCCAAGGCACACAAGTGA
		CTGTCTCGTCTGCTAGCCACCATCACCATCACCAC

299	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGAAGCGTGCAAG
	Sequence	CCGGAGGCTCTCTGAGGCTGAGCTGTGCCGCCTCTAGGTT
	Encoding	CACATACAGCAGCTACTGCATGGGCTGGTTCAGACAAGCC
	SEQ ID NO:	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGCATCGATAGCG
	201	ATGGCTCCACTAGCTACACTGACAGCGTGAAGGGAAGGTT
		CACTATCAGCAAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACAGCCATGTACT
		ACTGTGCCCTCGATCTGATGAGCACAGTGGTGCCCGGCTT
		CTGTGGCTTTCTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGCGGAGGATCCC
		AAGTGCAGCTGCAAGAGTCCGGAGGAGGAAGCGTGCAAGC
		CGGCGGATCTCTGAGACTGAGCTGTGCCGCCTCTAGGTAC
		ACTTACAACAGCTACTGCATGGGCTGGTTCAGACAAGCCC
		CCGGCAAGGAAAGAGAGGGCGTGGCCACTATCGATAGCGA
		CGGCATGACTAGGTACGCTGATAGCGTCAAGGGAAGGTTC
		ACAATCTCCAAGGACAATGCTAAGAACACTCTGTACCTCC
		AGATGAACTCTCTGAAGCCAGAGGACACAGCCATGTACTA
		CTGCGCTGCCGATGCCGACTGCACTATCGCCGCCATGACT
		ACTAATCCTCTGGGCCAAGGCACACAAGTGACTGTCTCGT
		CTGCTAGCCACCATCACCATCACCAC

300	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCCGCCTCTAGGTTCACATACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	202	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGC
		GGAGGATCCCAAGTGCAGCTGCAAGAGTCC
		GGCGGAGGCAGCGTCCAAGCCGGAGGATCT
		CTGAGGCTGAGCTGTACAGTGAGCAGATAC
		ACTGCCAGCGTGAACTACATGGGCTGGTTC
		AGACAAGCCCCCGGCAAAGAGAGAGAGGGC
		GTGGCCACAATCTTCACTGGCGCCGGCACA
		ACATACTACGCCAACTCCGTCAAGGGAAGG
		TTCACAATCTCTAGGGACAACGCCAAGAAC
		ACTGCCTATCTGCAGATGAACTCCCTCAAG
		CCAGAGGACACTGCCATCTACTACTGCGCC
		GTGGATTTCAGAGGCGGACTGCTGTATAGG
		CCAGCCTACGAGTACACTTATAGGGGCCAA
		GGCACACAAGTGACAGTCTCGTCTGCTAGC
		CACCATCACCATCACCAC

301	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCCGCCTCTAGGTTCACATACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	203	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGC
		GGAGGATCCCAAGTGCAGCTGCAAGAGAGC
		GGAGGAGGCAGCGTCGAAGCTGGAGGATCT
		CTGAGGCTGAGCTGTGCTGCCAGCGGCTAC
		ACTCACAGCAGCTACTGTATGGGCTGGTTC
		AGACAAGCCCCCGGCAAGGAGAGGGAAGGC
		GTGGCTGCCATCGACGTGGATGGCAGCACT
		ACTTACGCCGACAGCGTGAAGGGAAGGTTC
		ACTATCAGCAAGGACAACGCCAAGAACACA
		CTCTATCTGCAGATGAACAGCCTCAAGCCA
		GAGGACACTGGCATGTACTACTGCGCCGCC
		GAGTTCGCCGATTGCAGCAGCAACTACTTT
		CTGCCTCCCGGCGCCGTCAGATATTGGGGC
		CAAGGCACTCAAGTGACAGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

302	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCCGCCTCTAGGTTCACATACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	204	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGC
		GGAGGATCCCAAGTGCAGCTGCAAGAGAGC
		GGAGGAGGAAGCGTCCAAGCCGGAGGATCT
		CTGAGACTGAGCTGCGCCGCTAGTGGCTAC
		TCCTACAGCAGCTACTGCATGGGCTGGTTT
		AGGCAAGCCCCCGGCAAGGAGAGAGAAGGC
		GTGGCCACTATCGACAGCGACGGCATGACA
		AGGTACGCCGACAGCGTGAAGGGAAGGTTC
		ACAATCAGCAAGGACAACGCCAAGAACACA
		CTGTATCTGCAGATGAACTCTCTGAAGCCA
		GAGGACACTGCCATGTACTACTGTGCCGCT
		CCTCTGTACGACTGTGATAGCGGCGCTGTG
		GGCAGAAATCCACCTTATTGGGGCCAAGGC
		ACTCAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

303	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCCGCCTCTAGGTTCACATACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	205	CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGAGCGGC
		GGAGGATCCCAAGTGCAGCTGCAAGAGAGC
		GGAGGCGGCAGCGTGCAGACTGGAGGCTCT
		CTGAGACTGAGCTGTGCTGCCAGCGGCTAC
		ACTTATCTGAGGGGCTGTATGGGCTGGTTT
		AGGCAAGCCCCCGGCAAGGAGAGAGAGGGC
		GTGGCCGTCATGGATGTGGTGGGCGATAGG
		AGAAGCTACATCGACAGCGTGAAGGGAAGG
		TTCACAATCTCTAGGGACAATGCCGCCAAC
		AGCGTCTATCTGCAGATGGACAATCTGAAG
		CCAGAGGACACAGCCATGTACTACTGCACT
		GCCGGCCCTAACTGTGTGGGCTGGAGAAGC
		GGACTGGATTACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

304	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	206	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGCGGAGGAAGCGTGCAAGCTGGA
		GGCTCTCTGAGGCTGAGCTGTGCTGCCAGC
		GGCTACACTTATAGCAGCGGCTGTATGGGC
		TGGTTCAGACAAGCCCCCGGCAAGGAAAGG
		GAAGCCGTGGCCGCCATCAATTCCGATGGC
		AGCACAAGCTACGCCGACAGCGTGAAGGGA
		AGGTTCACAATCAGCAAGGACAACGCCAAG
		AACACACTCTATCTGCAGATGAACTCTCTG
		AAGCCAGAGGACACAGCCATGTACTACTGC
		GCCGCTGAGCCTTACTGTAGCGGCGGCTAC
		CCAAGATGGAGCGTCGCTGAGTTCGGCTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

305	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	207	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGCAGCGTCCAAGCCGGA
		GGCTCTCTGAGGCTGAGCTGTGCTGCCAGC
		GGCTACACTTACAGCAGCTACTGCATGGGC
		TGGTTCAGACAAGCCCCCGGCAAGGAGAGA
		GAGGGCGTGGCTCACATCGACAGCGACGGC
		TCCACAAGCTACGCCGATAGCGTGAAGGGA
		AGGTTCACAATCTCCAAGGACAACGCCAAG
		AACACTCTGTACCTCCAGATGAACTCTCTG
		AAGCCAGAGGACACTGCCATGTACTACTGT
		GCCGCCGATCCAATTCCCGGCCCCGGCTAC
		TGCGATGGCGGCCCTAACAAGTACTGGGGC
		CAAGGCACACAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

306	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	208	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGTCCGGAGGAGGAAGCGTGCAAGCCGGC
		GGATCTCTGAGACTGAGCTGTGCCGCCTCT
		AGGTACACTTACAACAGCTACTGCATGGGC
		TGGTTCAGACAAGCCCCCGGCAAGGAAAGA
		GAGGGCGTGGCCACTATCGATAGCGACGGC
		ATGACTAGGTACGCTGATAGCGTCAAGGGA
		AGGTTCACAATCTCCAAGGACAATGCTAAG
		AACACTCTGTACCTCCAGATGAACTCTCTG
		AAGCCAGAGGACACAGCCATGTACTACTGC
		GCTGCCGATGCCGACTGCACTATCGCCGCC
		ATGACTACTAATCCTCTGGGCCAAGGCACA
		CAAGTGACTGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

307	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	209	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGTCCGGCGGAGGCAGCGTCCAAGCCGGA
		GGATCTCTGAGGCTGAGCTGTACAGTGAGC
		AGATACACTGCCAGCGTGAACTACATGGGC
		TGGTTCAGACAAGCCCCCGGCAAAGAGAGA
		GAGGGCGTGGCCACAATCTTCACTGGCGCC
		GGCACAACATACTACGCCAACTCCGTCAAG
		GGAAGGTTCACAATCTCTAGGGACAACGCC
		AAGAACACTGCCTATCTGCAGATGAACTCC
		CTCAAGCCAGAGGACACTGCCATCTACTAC
		TGCGCCGTGGATTTCAGAGGCGGACTGCTG
		TATAGGCCAGCCTACGAGTACACTTATAGG
		GGCCAAGGCACACAAGTGACAGTCTCGTCT
		GCTAGCCACCATCACCATCACCAC

308	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	210	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGCAGCGTCGAAGCTGGA
		GGATCTCTGAGGCTGAGCTGTGCTGCCAGC
		GGCTACACTCACAGCAGCTACTGTATGGGC
		TGGTTCAGACAAGCCCCCGGCAAGGAGAGG
		GAAGGCGTGGCTGCCATCGACGTGGATGGC
		AGCACTACTTACGCCGACAGCGTGAAGGGA
		AGGTTCACTATCAGCAAGGACAACGCCAAG
		AACACACTCTATCTGCAGATGAACAGCCTC
		AAGCCAGAGGACACTGGCATGTACTACTGC
		GCCGCCGAGTTCGCCGATTGCAGCAGCAAC
		TACTTTCTGCCTCCCGGCGCCGTCAGATAT
		TGGGGCCAAGGCACTCAAGTGACAGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

309	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	211	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTCCAAGCCGGA
		GGATCTCTGAGACTGAGCTGCGCCGCTAGT
		GGCTACTCCTACAGCAGCTACTGCATGGGC
		TGGTTTAGGCAAGCCCCCGGCAAGGAGAGA
		GAAGGCGTGGCCACTATCGACAGCGACGGC
		ATGACAAGGTACGCCGACAGCGTGAAGGGA
		AGGTTCACAATCAGCAAGGACAACGCCAAG
		AACACACTGTATCTGCAGATGAACTCTCTG
		AAGCCAGAGGACACTGCCATGTACTACTGT
		GCCGCTCCTCTGTACGACTGTGATAGCGGC
		GCTGTGGGCAGAAATCCACCTTATTGGGGC
		CAAGGCACTCAAGTGACAGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

310	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	ATGTACTGCATGGGCTGGTTCAGACAAGCC
	212	CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGCGGCAGCGTGCAGACTGGA
		GGCTCTCTGAGACTGAGCTGTGCTGCCAGC
		GGCTACACTTATCTGAGGGGCTGTATGGGC
		TGGTTTAGGCAAGCCCCCGGCAAGGAGAGA
		GAGGGCGTGGCCGTCATGGATGTGGTGGGC
		GATAGGAGAAGCTACATCGACAGCGTGAAG
		GGAAGGTTCACAATCTCTAGGGACAATGCC
		GCCAACAGCGTCTATCTGCAGATGGACAAT
		CTGAAGCCAGAGGACACAGCCATGTACTAC
		TGCACTGCCGGCCCTAACTGTGTGGGCTGG
		AGAAGCGGACTGGATTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

311	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	213	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGCGGAGGAAGCGTG
		CAAGCTGGAGGCTCTCTGAGGCTGAGCTGT
		GCTGCCAGCGGCTACACTTATAGCAGCGGC
		TGTATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAAAGGGAAGCCGTGGCCGCCATCAAT
		TCCGATGGCAGCACAAGCTACGCCGACAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGCCAAGAACACACTCTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGCGCCGCTGAGCCTTACTGTAGC
		GGCGGCTACCCAAGATGGAGCGTCGCTGAG
		TTCGGCTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

312	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	214	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGCAGCGTC
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GCTGCCAGCGGCTACACTTACAGCAGCTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAGAGAGAGGGCGTGGCTCACATCGAC
		AGCGACGGCTCCACAAGCTACGCCGATAGC
		GTGAAGGGAAGGTTCACAATCTCCAAGGAC
		AACGCCAAGAACACTCTGTACCTCCAGATG
		AACTCTCTGAAGCCAGAGGACACTGCCATG
		TACTACTGTGCCGCCGATCCAATTCCCGGC
		CCCGGCTACTGCGATGGCGGCCCTAACAAG
		TACTGGGGCCAAGGCACACAAGTGACTGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

313	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	215	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGTCCGGAGGAGGAAGCGTG
		CAAGCCGGCGGATCTCTGAGACTGAGCTGT
		GCCGCCTCTAGGTACACTTACAACAGCTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAAAGAGAGGGCGTGGCCACTATCGAT
		AGCGACGGCATGACTAGGTACGCTGATAGC
		GTCAAGGGAAGGTTCACAATCTCCAAGGAC
		AATGCTAAGAACACTCTGTACCTCCAGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGCGCTGCCGATGCCGACTGCACT
		ATCGCCGCCATGACTACTAATCCTCTGGGC
		CAAGGCACACAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

314	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	216	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGTCCGGCGGAGGCAGCGTC
		CAAGCCGGAGGATCTCTGAGGCTGAGCTGT
		ACAGTGAGCAGATACACTGCCAGCGTGAAC
		TACATGGGCTGGTTCAGACAAGCCCCCGGC
		AAAGAGAGAGAGGGCGTGGCCACAATCTTC
		ACTGGCGCCGGCACAACATACTACGCCAAC
		TCCGTCAAGGGAAGGTTCACAATCTCTAGG
		GACAACGCCAAGAACACTGCCTATCTGCAG
		ATGAACTCCCTCAAGCCAGAGGACACTGCC
		ATCTACTACTGCGCCGTGGATTTCAGAGGC
		GGACTGCTGTATAGGCCAGCCTACGAGTAC
		ACTTATAGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

315	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	217	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGCAGCGTC
		GAAGCTGGAGGATCTCTGAGGCTGAGCTGT
		GCTGCCAGCGGCTACACTCACAGCAGCTAC
		TGTATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAGAGGGAAGGCGTGGCTGCCATCGAC
		GTGGATGGCAGCACTACTTACGCCGACAGC
		GTGAAGGGAAGGTTCACTATCAGCAAGGAC
		AACGCCAAGAACACACTCTATCTGCAGATG
		AACAGCCTCAAGCCAGAGGACACTGGCATG
		TACTACTGCGCCGCCGAGTTCGCCGATTGC
		AGCAGCAACTACTTTCTGCCTCCCGGCGCC
		GTCAGATATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

316	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	218	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTC
		CAAGCCGGAGGATCTCTGAGACTGAGCTGC
		GCCGCTAGTGGCTACTCCTACAGCAGCTAC
		TGCATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAGGAGAGAGAAGGCGTGGCCACTATCGAC
		AGCGACGGCATGACAAGGTACGCCGACAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGCCAAGAACACACTGTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACTGCCATG
		TACTACTGTGCCGCTCCTCTGTACGACTGT
		GATAGCGGCGCTGTGGGCAGAAATCCACCT
		TATTGGGGCCAAGGCACTCAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

317	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCTGTGAGCGGCTACGCCTACTCC
	SEQ ID NO:	ACATACTGCATGGGCTGGTTTAGGCAAGCC
	219	CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGCGGCAGCGTG
		CAGACTGGAGGCTCTCTGAGACTGAGCTGT
		GCTGCCAGCGGCTACACTTATCTGAGGGGC
		TGTATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAGGAGAGAGAGGGCGTGGCCGTCATGGAT
		GTGGTGGGCGATAGGAGAAGCTACATCGAC
		AGCGTGAAGGGAAGGTTCACAATCTCTAGG
		GACAATGCCGCCAACAGCGTCTATCTGCAG
		ATGGACAATCTGAAGCCAGAGGACACAGCC
		ATGTACTACTGCACTGCCGGCCCTAACTGT
		GTGGGCTGGAGAAGCGGACTGGATTACTGG
		GGCCAAGGCACACAAGTGACAGTCTCGTCT
		GCTAGCCACCATCACCATCACCAC

318	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	220	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGCGGA
		GGAAGCGTGCAAGCTGGAGGCTCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTTAT
		AGCAGCGGCTGTATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAAAGGGAAGCCGTGGCC
		GCCATCAATTCCGATGGCAGCACAAGCTAC
		GCCGACAGCGTGAAGGGAAGGTTCACAATC
		AGCAAGGACAACGCCAAGAACACACTCTAT
		CTGCAGATGAACTCTCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCGCCGCTGAGCCT
		TACTGTAGCGGCGGCTACCCAAGATGGAGC
		GTCGCTGAGTTCGGCTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

319	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	221	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGCAGCGTCCAAGCCGGAGGCTCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTTAC
		AGCAGCTACTGCATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAGAGAGAGGGCGTGGCT
		CACATCGACAGCGACGGCTCCACAAGCTAC
		GCCGATAGCGTGAAGGGAAGGTTCACAATC
		TCCAAGGACAACGCCAAGAACACTCTGTAC
		CTCCAGATGAACTCTCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCCGCCGATCCA
		ATTCCCGGCCCCGGCTACTGCGATGGCGGC
		CCTAACAAGTACTGGGGCCAAGGCACACAA
		GTGACTGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

320	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	222	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGTCCGGAGGA
		GGAAGCGTGCAAGCCGGCGGATCTCTGAGA
		CTGAGCTGTGCCGCCTCTAGGTACACTTAC
		AACAGCTACTGCATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAAAGAGAGGGCGTGGCC
		ACTATCGATAGCGACGGCATGACTAGGTAC
		GCTGATAGCGTCAAGGGAAGGTTCACAATC
		TCCAAGGACAATGCTAAGAACACTCTGTAC
		CTCCAGATGAACTCTCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCGCTGCCGATGCC
		GACTGCACTATCGCCGCCATGACTACTAAT
		CCTCTGGGCCAAGGCACACAAGTGACTGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

321	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	223	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGTCCGGCGGA
		GGCAGCGTCCAAGCCGGAGGATCTCTGAGG
		CTGAGCTGTACAGTGAGCAGATACACTGCC
		AGCGTGAACTACATGGGCTGGTTCAGACAA
		GCCCCCGGCAAAGAGAGAGAGGGCGTGGCC
		ACAATCTTCACTGGCGCCGGCACAACATAC
		TACGCCAACTCCGTCAAGGGAAGGTTCACA
		ATCTCTAGGGACAACGCCAAGAACACTGCC
		TATCTGCAGATGAACTCCCTCAAGCCAGAG
		GACACTGCCATCTACTACTGCGCCGTGGAT
		TTCAGAGGCGGACTGCTGTATAGGCCAGCC
		TACGAGTACACTTATAGGGGCCAAGGCACA
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

322	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	224	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGCAGCGTCGAAGCTGGAGGATCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTCAC
		AGCAGCTACTGTATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAGAGGGAAGGCGTGGCT
		GCCATCGACGTGGATGGCAGCACTACTTAC
		GCCGACAGCGTGAAGGGAAGGTTCACTATC
		AGCAAGGACAACGCCAAGAACACACTCTAT
		CTGCAGATGAACAGCCTCAAGCCAGAGGAC
		ACTGGCATGTACTACTGCGCCGCCGAGTTC
		GCCGATTGCAGCAGCAACTACTTTCTGCCT
		CCCGGCGCCGTCAGATATTGGGGCCAAGGC
		ACTCAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

323	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	225	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGAAGCGTCCAAGCCGGAGGATCTCTGAGA
		CTGAGCTGCGCCGCTAGTGGCTACTCCTAC
		AGCAGCTACTGCATGGGCTGGTTTAGGCAA
		GCCCCCGGCAAGGAGAGAGAAGGCGTGGCC
		ACTATCGACAGCGACGGCATGACAAGGTAC
		GCCGACAGCGTGAAGGGAAGGTTCACAATC
		AGCAAGGACAACGCCAAGAACACACTGTAT
		CTGCAGATGAACTCTCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCCGCTCCTCTG
		TACGACTGTGATAGCGGCGCTGTGGGCAGA
		AATCCACCTTATTGGGGCCAAGGCACTCAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

324	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTACAGTGTCCGGCTACACTTACAGC
	SEQ ID NO:	TCCAATTGCATGGGCTGGTTTAGGCAAGCC
	226	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGC
		GGCAGCGTGCAGACTGGAGGCTCTCTGAGA
		CTGAGCTGTGCTGCCAGCGGCTACACTTAT
		CTGAGGGGCTGTATGGGCTGGTTTAGGCAA
		GCCCCCGGCAAGGAGAGAGAGGGCGTGGCC
		GTCATGGATGTGGTGGGCGATAGGAGAAGC
		TACATCGACAGCGTGAAGGGAAGGTTCACA
		ATCTCTAGGGACAATGCCGCCAACAGCGTC
		TATCTGCAGATGGACAATCTGAAGCCAGAG
		GACACAGCCATGTACTACTGCACTGCCGGC
		CCTAACTGTGTGGGCTGGAGAAGCGGACTG
		GATTACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

325	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	227	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
		AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
		AGCTGTGCTGCCAGCGGCTACACTTATAGC
		AGCGGCTGTATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

326	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	228	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
		AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGCTGCCAGCGGCTACACTTACAGC
		AGCTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

327	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	229	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
		AGCGTGCAAGCCGGCGGATCTCTGAGACTG
		AGCTGTGCCGCCTCTAGGTACACTTACAAC
		AGCTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

328	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	230	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
		AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
		AGCTGTACAGTGAGCAGATACACTGCCAGC
		GTGAACTACATGGGCTGGTTCAGACAAGCC
		CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

329	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	231	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
		AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
		AGCTGTGCTGCCAGCGGCTACACTCACAGC
		AGCTACTGTATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

330	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	232	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTCCAAGCCGGAGGATCTCTGAGACTG
		AGCTGCGCCGCTAGTGGCTACTCCTACAGC
		AGCTACTGCATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

331	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGGAGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTTAGGCAAGTG
	233	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
		AGCGTGCAGACTGGAGGCTCTCTGAGACTG
		AGCTGTGCTGCCAGCGGCTACACTTATCTG
		AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

332	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	234	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGCGGA
		GGAAGCGTGCAAGCTGGAGGCTCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTTAT
		AGCAGCGGCTGTATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAAAGGGAAGCCGTGGCC
		GCCATCAATTCCGATGGCAGCACAAGCTAC
		GCCGACAGCGTGAAGGGAAGGTTCACAATC
		AGCAAGGACAACGCCAAGAACACACTCTAT
		CTGCAGATGAACTCTCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCGCCGCTGAGCCT
		TACTGTAGCGGCGGCTACCCAAGATGGAGC
		GTCGCTGAGTTCGGCTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

333	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	235	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGCAGCGTCCAAGCCGGAGGCTCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTTAC
		AGCAGCTACTGCATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAGAGAGAGGGCGTGGCT
		CACATCGACAGCGACGGCTCCACAAGCTAC
		GCCGATAGCGTGAAGGGAAGGTTCACAATC
		TCCAAGGACAACGCCAAGAACACTCTGTAC
		CTCCAGATGAACTCTCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCCGCCGATCCA
		ATTCCCGGCCCCGGCTACTGCGATGGCGGC
		CCTAACAAGTACTGGGGCCAAGGCACACAA
		GTGACTGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

334	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	236	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGTCCGGAGGA
		GGAAGCGTGCAAGCCGGCGGATCTCTGAGA
		CTGAGCTGTGCCGCCTCTAGGTACACTTAC
		AACAGCTACTGCATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAAAGAGAGGGCGTGGCC
		ACTATCGATAGCGACGGCATGACTAGGTAC
		GCTGATAGCGTCAAGGGAAGGTTCACAATC
		TCCAAGGACAATGCTAAGAACACTCTGTAC
		CTCCAGATGAACTCTCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCGCTGCCGATGCC
		GACTGCACTATCGCCGCCATGACTACTAAT
		CCTCTGGGCCAAGGCACACAAGTGACTGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

335	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	237	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGTCCGGCGGA
		GGCAGCGTCCAAGCCGGAGGATCTCTGAGG
		CTGAGCTGTACAGTGAGCAGATACACTGCC
		AGCGTGAACTACATGGGCTGGTTCAGACAA
		GCCCCCGGCAAAGAGAGAGAGGGCGTGGCC
		ACAATCTTCACTGGCGCCGGCACAACATAC
		TACGCCAACTCCGTCAAGGGAAGGTTCACA
		ATCTCTAGGGACAACGCCAAGAACACTGCC
		TATCTGCAGATGAACTCCCTCAAGCCAGAG
		GACACTGCCATCTACTACTGCGCCGTGGAT
		TTCAGAGGCGGACTGCTGTATAGGCCAGCC
		TACGAGTACACTTATAGGGGCCAAGGCACA
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

336	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	238	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGCAGCGTCGAAGCTGGAGGATCTCTGAGG
		CTGAGCTGTGCTGCCAGCGGCTACACTCAC
		AGCAGCTACTGTATGGGCTGGTTCAGACAA
		GCCCCCGGCAAGGAGAGGGAAGGCGTGGCT
		GCCATCGACGTGGATGGCAGCACTACTTAC
		GCCGACAGCGTGAAGGGAAGGTTCACTATC
		AGCAAGGACAACGCCAAGAACACACTCTAT
		CTGCAGATGAACAGCCTCAAGCCAGAGGAC
		ACTGGCATGTACTACTGCGCCGCCGAGTTC
		GCCGATTGCAGCAGCAACTACTTTCTGCCT
		CCCGGCGCCGTCAGATATTGGGGCCAAGGC
		ACTCAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

337	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	239	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGA
		GGAAGCGTCCAAGCCGGAGGATCTCTGAGA
		CTGAGCTGCGCCGCTAGTGGCTACTCCTAC
		AGCAGCTACTGCATGGGCTGGTTTAGGCAA
		GCCCCCGGCAAGGAGAGAGAAGGCGTGGCC
		ACTATCGACAGCGACGGCATGACAAGGTAC
		GCCGACAGCGTGAAGGGAAGGTTCACAATC
		AGCAAGGACAACGCCAAGAACACACTGTAT
		CTGCAGATGAACTCTCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCCGCTCCTCTG
		TACGACTGTGATAGCGGCGCTGTGGGCAGA
		AATCCACCTTATTGGGGCCAAGGCACTCAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

338	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCCGCCAGCGGCTACTCCAACTGC
	SEQ ID NO:	AGCTACGACATGACTTGGTATAGGCAAGCC
	240	CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGAGCGGCGGAGGA
		TCCCAAGTGCAGCTGCAAGAGAGCGGAGGC
		GGCAGCGTGCAGACTGGAGGCTCTCTGAGA
		CTGAGCTGTGCTGCCAGCGGCTACACTTAT
		CTGAGGGGCTGTATGGGCTGGTTTAGGCAA
		GCCCCCGGCAAGGAGAGAGAGGGCGTGGCC
		GTCATGGATGTGGTGGGCGATAGGAGAAGC
		TACATCGACAGCGTGAAGGGAAGGTTCACA
		ATCTCTAGGGACAATGCCGCCAACAGCGTC
		TATCTGCAGATGGACAATCTGAAGCCAGAG
		GACACAGCCATGTACTACTGCACTGCCGGC
		CCTAACTGTGTGGGCTGGAGAAGCGGACTG
		GATTACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

339	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	241	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGACTG
		AGCTGTGCCGCCTCTAGGTATCTGTACAGC
		ATCGACTACATGGCTTGGTTCAGACAGAGC
		CCCGGCAAGGAGAGGGAGCCAGTGGCTGTC
		ATCTACACTGCCTCCGGCGCCACATTCTAT
		CCAGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGAC
		ACTGCCATGTACTACTGTGCCGCCGTGAGG
		AAGACAGATAGCTACCTCTTCGACGCCCAG
		AGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

340	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	242	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGCCGCCTCTAGGTTCACATACAGC
		AGCTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

341	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	243	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
		AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGCTGCCAGCGGCTACACTTACAGC
		ATGTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

342	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	244	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
		AGCGTGCAAGCCGGAGGATCTCTGAGACTG
		AGCTGCGCTGTGAGCGGCTACGCCTACTCC
		ACATACTGCATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

343	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	245	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTACAGTGTCCGGCTACACTTACAGC
		TCCAATTGCATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

344	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	246	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGGAGCCAGCGGCTACACTTACAGC
		AGCTACTGTATGGGCTGGTTTAGGCAAGTG
		CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

345	DNA	CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
	Sequence	AGCGTGCAAGCTGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATAGC
	SEQ ID NO:	AGCGGCTGTATGGGCTGGTTCAGACAAGCC
	247	CCCGGCAAGGAAAGGGAAGCCGTGGCCGCC
		ATCAATTCCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGAGCCTTAC
		TGTAGCGGCGGCTACCCAAGATGGAGCGTC
		GCTGAGTTCGGCTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
		AGCTGTGCCGCCAGCGGCTACTCCAACTGC
		AGCTACGACATGACTTGGTATAGGCAAGCC
		CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

346	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	248	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGACTGAGCTGT
		GCCGCCTCTAGGTATCTGTACAGCATCGAC
		TACATGGCTTGGTTCAGACAGAGCCCCGGC
		AAGGAGAGGGAGCCAGTGGCTGTCATCTAC
		ACTGCCTCCGGCGCCACATTCTATCCAGAT
		AGCGTGAAGGGAAGGTTCACTATCAGCCAA
		GATAACGCCAAGATGACAGTGTATCTGCAG
		ATGAACTCTCTGAAGAGCGAGGACACTGCC
		ATGTACTACTGTGCCGCCGTGAGGAAGACA
		GATAGCTACCTCTTCGACGCCCAGAGCTTC
		ACATACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

347	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	249	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GCCGCCTCTAGGTTCACATACAGCAGCTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAAGAGAGAGAAGGCGTGGCCAGCATCGAT
		AGCGATGGCTCCACTAGCTACACTGACAGC
		GTGAAGGGAAGGTTCACTATCAGCAAGGAC
		AACGCCAAGAACACTCTGTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGTGCCCTCGATCTGATGAGCACA
		GTGGTGCCCGGCTTCTGTGGCTTTCTGCTG
		AGCGCTGGCATGGATTACTGGGGCAAGGGC
		ACTCAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

348	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	250	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGTCCGGAGGAGGCAGCGTC
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GCTGCCAGCGGCTACACTTACAGCATGTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAAAGAGAGGGCGTGGCCCAGATCAAT
		AGCGATGGCAGCACAAGCTACGCCGACAGC
		GTGAAGGGAAGGTTCACTATCTCCAAGGAC
		AACGCCAAGAACACTCTGTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACTGCCATG
		TACTACTGCGCTGCCGATTCTAGGGTGTAC
		GGCGGCAGCTGGTATGAGAGGCTCTGCGGC
		CCTTACACATACGAGTACAACTACTGGGGC
		CAAGGCACACAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

349	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	251	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGCGGAGGAAGCGTG
		CAAGCCGGAGGATCTCTGAGACTGAGCTGC
		GCTGTGAGCGGCTACGCCTACTCCACATAC
		TGCATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAAGAGAGAGAGGGCGTGGCTGCTATCGAT
		AGCGGCGGCAGCACAAGCTACGCCGATAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGCCAAGAACACACTGTATCTGAGGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGTGCTGCTGTGCCTCCTCCTCCA
		GATGGCGGCAGCTGTCTGTTTCTGGGACCA
		GAGATCAAGGTCAGCAAGGCCGATTTTAGG
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

350	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	252	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		ACAGTGTCCGGCTACACTTACAGCTCCAAT
		TGCATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAGGAAAGAGAGGGCGTGGCCACTATCTAC
		ACTGGCGGCGGCAACACATACTACGCCGAT
		AGCGTGAAGGGAAGGTTCACTATCAGCCAA
		GATAACGCCAAGAACACAGTGTATCTGCAG
		ATGAACAATCTGAAGCCAGAGGACACTGCC
		ATGTACTACTGTGCTGCTGAGCCACTGTCT
		AGGGTGTACGGCGGCAGCTGCCCAACTCCT
		ACATTCGACTACTGGGGCCAAGGCACACAA
		GTGACTGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

351	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	253	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTC
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GGAGCCAGCGGCTACACTTACAGCAGCTAC
		TGTATGGGCTGGTTTAGGCAAGTGCCCGGC
		AAGGAGAGAGAGGGCGTGGCCGTGATCGAT
		TCCGATGGCAGCACAAGCTACGCTGACAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGGCAAGAACACACTCTATCTGCAGATG
		AACAGCCTCAAGCCAGAGGACACAGCCATG
		TACTACTGCGCCGCTGATCTGGGCCACTAT
		AGGCCTCCTTGTGGCGTGCTGTATCTGGGC
		ATGGATTACTGGGGCAAGGGCACACAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

352	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	254	CCCGGCAAGGAGAGAGAGGGCGTGGCTCAC
		ATCGACAGCGACGGCTCCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCTCC
		AAGGACAACGCCAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCCGATCCAATT
		CCCGGCCCCGGCTACTGCGATGGCGGCCCT
		AACAAGTACTGGGGCCAAGGCACACAAGTG
		ACTGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTC
		CAAGCCGGAGGCTCTCTGAGACTGAGCTGT
		GCCGCCAGCGGCTACTCCAACTGCAGCTAC
		GACATGACTTGGTATAGGCAAGCCCCCGGC
		AAGGAGAGGGAGTTCGTGTCCGCCATCCAC
		AGCGACGGCAGCACTAGATACGCCGACAGC
		GTGAAGGGAAGGTTCTTCATCAGCCAAGAT
		AACGCCAAGAACACAGTGTATCTGCAGATG
		AACTCCCTCAAGCCAGAGGACACTGCCATG
		TACTACTGCAAGACAGACCCACTGCACTGC
		AGAGCCCATGGCGGCAGCTGGTATAGCGTG
		AGGGCCAACTACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

353	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	255	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTGCAAGCCGGA
		GGCTCTCTGAGACTGAGCTGTGCCGCCTCT
		AGGTATCTGTACAGCATCGACTACATGGCT
		TGGTTCAGACAGAGCCCCGGCAAGGAGAGG
		GAGCCAGTGGCTGTCATCTACACTGCCTCC
		GGCGCCACATTCTATCCAGATAGCGTGAAG
		GGAAGGTTCACTATCAGCCAAGATAACGCC
		AAGATGACAGTGTATCTGCAGATGAACTCT
		CTGAAGAGCGAGGACACTGCCATGTACTAC
		TGTGCCGCCGTGAGGAAGACAGATAGCTAC
		CTCTTCGACGCCCAGAGCTTCACATACTGG
		GGCCAAGGCACACAAGTGACAGTCTCGTCT
		GCTAGCCACCATCACCATCACCAC

354	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	256	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTGCAAGCCGGA
		GGCTCTCTGAGGCTGAGCTGTGCCGCCTCT
		AGGTTCACATACAGCAGCTACTGCATGGGC
		TGGTTCAGACAAGCCCCCGGCAAAGAGAGA
		GAAGGCGTGGCCAGCATCGATAGCGATGGC
		TCCACTAGCTACACTGACAGCGTGAAGGGA
		AGGTTCACTATCAGCAAGGACAACGCCAAG
		AACACTCTGTATCTGCAGATGAACTCTCTG
		AAGCCAGAGGACACAGCCATGTACTACTGT
		GCCCTCGATCTGATGAGCACAGTGGTGCCC
		GGCTTCTGTGGCTTTCTGCTGAGCGCTGGC
		ATGGATTACTGGGGCAAGGGCACTCAAGTG
		ACTGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

355	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	257	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGTCCGGAGGAGGCAGCGTCCAAGCCGGA
		GGCTCTCTGAGGCTGAGCTGTGCTGCCAGC
		GGCTACACTTACAGCATGTACTGCATGGGC
		TGGTTCAGACAAGCCCCCGGCAAGGAAAGA
		GAGGGCGTGGCCCAGATCAATAGCGATGGC
		AGCACAAGCTACGCCGACAGCGTGAAGGGA
		AGGTTCACTATCTCCAAGGACAACGCCAAG
		AACACTCTGTATCTGCAGATGAACTCTCTG
		AAGCCAGAGGACACTGCCATGTACTACTGC
		GCTGCCGATTCTAGGGTGTACGGCGGCAGC
		TGGTATGAGAGGCTCTGCGGCCCTTACACA
		TACGAGTACAACTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

356	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	258	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGCGGAGGAAGCGTGCAAGCCGGA
		GGATCTCTGAGACTGAGCTGCGCTGTGAGC
		GGCTACGCCTACTCCACATACTGCATGGGC
		TGGTTTAGGCAAGCCCCCGGCAAAGAGAGA
		GAGGGCGTGGCTGCTATCGATAGCGGCGGC
		AGCACAAGCTACGCCGATAGCGTGAAGGGA
		AGGTTCACAATCAGCAAGGACAACGCCAAG
		AACACACTGTATCTGAGGATGAACTCTCTG
		AAGCCAGAGGACACAGCCATGTACTACTGT
		GCTGCTGTGCCTCCTCCTCCAGATGGCGGC
		AGCTGTCTGTTTCTGGGACCAGAGATCAAG
		GTCAGCAAGGCCGATTTTAGGTACTGGGGC
		CAAGGCACACAAGTGACAGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

357	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	259	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTGCAAGCCGGA
		GGCTCTCTGAGGCTGAGCTGTACAGTGTCC
		GGCTACACTTACAGCTCCAATTGCATGGGC
		TGGTTTAGGCAAGCCCCCGGCAAGGAAAGA
		GAGGGCGTGGCCACTATCTACACTGGCGGC
		GGCAACACATACTACGCCGATAGCGTGAAG
		GGAAGGTTCACTATCAGCCAAGATAACGCC
		AAGAACACAGTGTATCTGCAGATGAACAAT
		CTGAAGCCAGAGGACACTGCCATGTACTAC
		TGTGCTGCTGAGCCACTGTCTAGGGTGTAC
		GGCGGCAGCTGCCCAACTCCTACATTCGAC
		TACTGGGGCCAAGGCACACAAGTGACTGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

358	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	260	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTCCAAGCCGGA
		GGCTCTCTGAGGCTGAGCTGTGGAGCCAGC
		GGCTACACTTACAGCAGCTACTGTATGGGC
		TGGTTTAGGCAAGTGCCCGGCAAGGAGAGA
		GAGGGCGTGGCCGTGATCGATTCCGATGGC
		AGCACAAGCTACGCTGACAGCGTGAAGGGA
		AGGTTCACAATCAGCAAGGACAACGGCAAG
		AACACACTCTATCTGCAGATGAACAGCCTC
		AAGCCAGAGGACACAGCCATGTACTACTGC
		GCCGCTGATCTGGGCCACTATAGGCCTCCT
		TGTGGCGTGCTGTATCTGGGCATGGATTAC
		TGGGGCAAGGGCACACAAGTGACAGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

359	DNA	CAAGTGCAGCTGCAAGAGTCCGGAGGAGGA
	Sequence	AGCGTGCAAGCCGGCGGATCTCTGAGACTG
	Encoding	AGCTGTGCCGCCTCTAGGTACACTTACAAC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTCAGACAAGCC
	261	CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCGATAGCGACGGCATGACTAGGTACGCT
		GATAGCGTCAAGGGAAGGTTCACAATCTCC
		AAGGACAATGCTAAGAACACTCTGTACCTC
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGCGCTGCCGATGCCGAC
		TGCACTATCGCCGCCATGACTACTAATCCT
		CTGGGCCAAGGCACACAAGTGACTGTCTCG
		AGCGGCGGAGGATCCCAAGTGCAGCTGCAA
		GAGAGCGGAGGAGGAAGCGTCCAAGCCGGA
		GGCTCTCTGAGACTGAGCTGTGCCGCCAGC
		GGCTACTCCAACTGCAGCTACGACATGACT
		TGGTATAGGCAAGCCCCCGGCAAGGAGAGG
		GAGTTCGTGTCCGCCATCCACAGCGACGGC
		AGCACTAGATACGCCGACAGCGTGAAGGGA
		AGGTTCTTCATCAGCCAAGATAACGCCAAG
		AACACAGTGTATCTGCAGATGAACTCCCTC
		AAGCCAGAGGACACTGCCATGTACTACTGC
		AAGACAGACCCACTGCACTGCAGAGCCCAT
		GGCGGCAGCTGGTATAGCGTGAGGGCCAAC
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

360	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	262	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGAGGAGGAAGC
		GTGCAAGCCGGAGGCTCTCTGAGACTGAGC
		TGTGCCGCCTCTAGGTATCTGTACAGCATC
		GACTACATGGCTTGGTTCAGACAGAGCCCC
		GGCAAGGAGAGGGAGCCAGTGGCTGTCATC
		TACACTGCCTCCGGCGCCACATTCTATCCA
		GATAGCGTGAAGGGAAGGTTCACTATCAGC
		CAAGATAACGCCAAGATGACAGTGTATCTG
		CAGATGAACTCTCTGAAGAGCGAGGACACT
		GCCATGTACTACTGTGCCGCCGTGAGGAAG
		ACAGATAGCTACCTCTTCGACGCCCAGAGC
		TTCACATACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

361	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	263	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGAGGAGGAAGC
		GTGCAAGCCGGAGGCTCTCTGAGGCTGAGC
		TGTGCCGCCTCTAGGTTCACATACAGCAGC
		TACTGCATGGGCTGGTTCAGACAAGCCCCC
		GGCAAAGAGAGAGAAGGCGTGGCCAGCATC
		GATAGCGATGGCTCCACTAGCTACACTGAC
		AGCGTGAAGGGAAGGTTCACTATCAGCAAG
		GACAACGCCAAGAACACTCTGTATCTGCAG
		ATGAACTCTCTGAAGCCAGAGGACACAGCC
		ATGTACTACTGTGCCCTCGATCTGATGAGC
		ACAGTGGTGCCCGGCTTCTGTGGCTTTCTG
		CTGAGCGCTGGCATGGATTACTGGGGCAAG
		GGCACTCAAGTGACTGTCTCGTCTGCTAGC
		CACCATCACCATCACCAC

362	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	264	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGTCCGGAGGAGGCAGC
		GTCCAAGCCGGAGGCTCTCTGAGGCTGAGC
		TGTGCTGCCAGCGGCTACACTTACAGCATG
		TACTGCATGGGCTGGTTCAGACAAGCCCCC
		GGCAAGGAAAGAGAGGGCGTGGCCCAGATC
		AATAGCGATGGCAGCACAAGCTACGCCGAC
		AGCGTGAAGGGAAGGTTCACTATCTCCAAG
		GACAACGCCAAGAACACTCTGTATCTGCAG
		ATGAACTCTCTGAAGCCAGAGGACACTGCC
		ATGTACTACTGCGCTGCCGATTCTAGGGTG
		TACGGCGGCAGCTGGTATGAGAGGCTCTGC
		GGCCCTTACACATACGAGTACAACTACTGG
		GGCCAAGGCACACAAGTGACTGTCTCGTCT
		GCTAGCCACCATCACCATCACCAC

363	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	265	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGCGGAGGAAGC
		GTGCAAGCCGGAGGATCTCTGAGACTGAGC
		TGCGCTGTGAGCGGCTACGCCTACTCCACA
		TACTGCATGGGCTGGTTTAGGCAAGCCCCC
		GGCAAAGAGAGAGAGGGCGTGGCTGCTATC
		GATAGCGGCGGCAGCACAAGCTACGCCGAT
		AGCGTGAAGGGAAGGTTCACAATCAGCAAG
		GACAACGCCAAGAACACACTGTATCTGAGG
		ATGAACTCTCTGAAGCCAGAGGACACAGCC
		ATGTACTACTGTGCTGCTGTGCCTCCTCCT
		CCAGATGGCGGCAGCTGTCTGTTTCTGGGA
		CCAGAGATCAAGGTCAGCAAGGCCGATTTT
		AGGTACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

364	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	266	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGAGGAGGAAGC
		GTGCAAGCCGGAGGCTCTCTGAGGCTGAGC
		TGTACAGTGTCCGGCTACACTTACAGCTCC
		AATTGCATGGGCTGGTTTAGGCAAGCCCCC
		GGCAAGGAAAGAGAGGGCGTGGCCACTATC
		TACACTGGCGGCGGCAACACATACTACGCC
		GATAGCGTGAAGGGAAGGTTCACTATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACAATCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCTGCTGAGCCACTG
		TCTAGGGTGTACGGCGGCAGCTGCCCAACT
		CCTACATTCGACTACTGGGGCCAAGGCACA
		CAAGTGACTGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

365	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	267	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGAGGAGGAAGC
		GTCCAAGCCGGAGGCTCTCTGAGGCTGAGC
		TGTGGAGCCAGCGGCTACACTTACAGCAGC
		TACTGTATGGGCTGGTTTAGGCAAGTGCCC
		GGCAAGGAGAGAGAGGGCGTGGCCGTGATC
		GATTCCGATGGCAGCACAAGCTACGCTGAC
		AGCGTGAAGGGAAGGTTCACAATCAGCAAG
		GACAACGGCAAGAACACACTCTATCTGCAG
		ATGAACAGCCTCAAGCCAGAGGACACAGCC
		ATGTACTACTGCGCCGCTGATCTGGGCCAC
		TATAGGCCTCCTTGTGGCGTGCTGTATCTG
		GGCATGGATTACTGGGGCAAGGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

366	DNA	CAAGTGCAGCTGCAAGAGTCCGGCGGAGGC
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTACAGTGAGCAGATACACTGCCAGC
	SEQ ID NO:	GTGAACTACATGGGCTGGTTCAGACAAGCC
	268	CCCGGCAAAGAGAGAGAGGGCGTGGCCACA
		ATCTTCACTGGCGCCGGCACAACATACTAC
		GCCAACTCCGTCAAGGGAAGGTTCACAATC
		TCTAGGGACAACGCCAAGAACACTGCCTAT
		CTGCAGATGAACTCCCTCAAGCCAGAGGAC
		ACTGCCATCTACTACTGCGCCGTGGATTTC
		AGAGGCGGACTGCTGTATAGGCCAGCCTAC
		GAGTACACTTATAGGGGCCAAGGCACACAA
		GTGACAGTCTCGAGCGGCGGAGGATCCCAA
		GTGCAGCTGCAAGAGAGCGGAGGAGGAAGC
		GTCCAAGCCGGAGGCTCTCTGAGACTGAGC
		TGTGCCGCCAGCGGCTACTCCAACTGCAGC
		TACGACATGACTTGGTATAGGCAAGCCCCC
		GGCAAGGAGAGGGAGTTCGTGTCCGCCATC
		CACAGCGACGGCAGCACTAGATACGCCGAC
		AGCGTGAAGGGAAGGTTCTTCATCAGCCAA
		GATAACGCCAAGAACACAGTGTATCTGCAG
		ATGAACTCCCTCAAGCCAGAGGACACTGCC
		ATGTACTACTGCAAGACAGACCCACTGCAC
		TGCAGAGCCCATGGCGGCAGCTGGTATAGC
		GTGAGGGCCAACTACTGGGGCCAAGGCACA
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

367	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	269	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGACTG
		AGCTGTGCCGCCTCTAGGTATCTGTACAGC
		ATCGACTACATGGCTTGGTTCAGACAGAGC
		CCCGGCAAGGAGAGGGAGCCAGTGGCTGTC
		ATCTACACTGCCTCCGGCGCCACATTCTAT
		CCAGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGATGACAGTGTAT
		CTGCAGATGAACTCTCTGAAGAGCGAGGAC
		ACTGCCATGTACTACTGTGCCGCCGTGAGG
		AAGACAGATAGCTACCTCTTCGACGCCCAG
		AGCTTCACATACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

368	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	270	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGCCGCCTCTAGGTTCACATACAGC
		AGCTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAAGAGAGAGAAGGCGTGGCCAGC
		ATCGATAGCGATGGCTCCACTAGCTACACT
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCCCTCGATCTGATG
		AGCACAGTGGTGCCCGGCTTCTGTGGCTTT
		CTGCTGAGCGCTGGCATGGATTACTGGGGC
		AAGGGCACTCAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

369	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	271	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGTCCGGAGGAGGC
		AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGCTGCCAGCGGCTACACTTACAGC
		ATGTACTGCATGGGCTGGTTCAGACAAGCC
		CCCGGCAAGGAAAGAGAGGGCGTGGCCCAG
		ATCAATAGCGATGGCAGCACAAGCTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCTCC
		AAGGACAACGCCAAGAACACTCTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGCGCTGCCGATTCTAGG
		GTGTACGGCGGCAGCTGGTATGAGAGGCTC
		TGCGGCCCTTACACATACGAGTACAACTAC
		TGGGGCCAAGGCACACAAGTGACTGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

370	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	272	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGCGGAGGA
		AGCGTGCAAGCCGGAGGATCTCTGAGACTG
		AGCTGCGCTGTGAGCGGCTACGCCTACTCC
		ACATACTGCATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAAGAGAGAGAGGGCGTGGCTGCT
		ATCGATAGCGGCGGCAGCACAAGCTACGCC
		GATAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		AGGATGAACTCTCTGAAGCCAGAGGACACA
		GCCATGTACTACTGTGCTGCTGTGCCTCCT
		CCTCCAGATGGCGGCAGCTGTCTGTTTCTG
		GGACCAGAGATCAAGGTCAGCAAGGCCGAT
		TTTAGGTACTGGGGCCAAGGCACACAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

371	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	273	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTGCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTACAGTGTCCGGCTACACTTACAGC
		TCCAATTGCATGGGCTGGTTTAGGCAAGCC
		CCCGGCAAGGAAAGAGAGGGCGTGGCCACT
		ATCTACACTGGCGGCGGCAACACATACTAC
		GCCGATAGCGTGAAGGGAAGGTTCACTATC
		AGCCAAGATAACGCCAAGAACACAGTGTAT
		CTGCAGATGAACAATCTGAAGCCAGAGGAC
		ACTGCCATGTACTACTGTGCTGCTGAGCCA
		CTGTCTAGGGTGTACGGCGGCAGCTGCCCA
		ACTCCTACATTCGACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

372	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	274	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTCCAAGCCGGAGGCTCTCTGAGGCTG
		AGCTGTGGAGCCAGCGGCTACACTTACAGC
		AGCTACTGTATGGGCTGGTTTAGGCAAGTG
		CCCGGCAAGGAGAGAGAGGGCGTGGCCGTG
		ATCGATTCCGATGGCAGCACAAGCTACGCT
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGGCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACA
		GCCATGTACTACTGCGCCGCTGATCTGGGC
		CACTATAGGCCTCCTTGTGGCGTGCTGTAT
		CTGGGCATGGATTACTGGGGCAAGGGCACA
		CAAGTGACAGTCTCGTCTGCTAGCCACCAT
		CACCATCACCAC

373	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGC
	Sequence	AGCGTCGAAGCTGGAGGATCTCTGAGGCTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTCACAGC
	SEQ ID NO:	AGCTACTGTATGGGCTGGTTCAGACAAGCC
	275	CCCGGCAAGGAGAGGGAAGGCGTGGCTGCC
		ATCGACGTGGATGGCAGCACTACTTACGCC
		GACAGCGTGAAGGGAAGGTTCACTATCAGC
		AAGGACAACGCCAAGAACACACTCTATCTG
		CAGATGAACAGCCTCAAGCCAGAGGACACT
		GGCATGTACTACTGCGCCGCCGAGTTCGCC
		GATTGCAGCAGCAACTACTTTCTGCCTCCC
		GGCGCCGTCAGATATTGGGGCCAAGGCACT
		CAAGTGACAGTCTCGAGCGGCGGAGGATCC
		CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
		AGCGTCCAAGCCGGAGGCTCTCTGAGACTG
		AGCTGTGCCGCCAGCGGCTACTCCAACTGC
		AGCTACGACATGACTTGGTATAGGCAAGCC
		CCCGGCAAGGAGAGGGAGTTCGTGTCCGCC
		ATCCACAGCGACGGCAGCACTAGATACGCC
		GACAGCGTGAAGGGAAGGTTCTTCATCAGC
		CAAGATAACGCCAAGAACACAGTGTATCTG
		CAGATGAACTCCCTCAAGCCAGAGGACACT
		GCCATGTACTACTGCAAGACAGACCCACTG
		CACTGCAGAGCCCATGGCGGCAGCTGGTAT
		AGCGTGAGGGCCAACTACTGGGGCCAAGGC
		ACACAAGTGACAGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

374	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	276	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGACTGAGCTGT
		GCCGCCTCTAGGTATCTGTACAGCATCGAC
		TACATGGCTTGGTTCAGACAGAGCCCCGGC
		AAGGAGAGGGAGCCAGTGGCTGTCATCTAC
		ACTGCCTCCGGCGCCACATTCTATCCAGAT
		AGCGTGAAGGGAAGGTTCACTATCAGCCAA
		GATAACGCCAAGATGACAGTGTATCTGCAG
		ATGAACTCTCTGAAGAGCGAGGACACTGCC
		ATGTACTACTGTGCCGCCGTGAGGAAGACA
		GATAGCTACCTCTTCGACGCCCAGAGCTTC
		ACATACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

375	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	277	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GCCGCCTCTAGGTTCACATACAGCAGCTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAAGAGAGAGAAGGCGTGGCCAGCATCGAT
		AGCGATGGCTCCACTAGCTACACTGACAGC
		GTGAAGGGAAGGTTCACTATCAGCAAGGAC
		AACGCCAAGAACACTCTGTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGTGCCCTCGATCTGATGAGCACA
		GTGGTGCCCGGCTTCTGTGGCTTTCTGCTG
		AGCGCTGGCATGGATTACTGGGGCAAGGGC
		ACTCAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

376	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	278	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGTCCGGAGGAGGCAGCGTC
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GCTGCCAGCGGCTACACTTACAGCATGTAC
		TGCATGGGCTGGTTCAGACAAGCCCCCGGC
		AAGGAAAGAGAGGGCGTGGCCCAGATCAAT
		AGCGATGGCAGCACAAGCTACGCCGACAGC
		GTGAAGGGAAGGTTCACTATCTCCAAGGAC
		AACGCCAAGAACACTCTGTATCTGCAGATG
		AACTCTCTGAAGCCAGAGGACACTGCCATG
		TACTACTGCGCTGCCGATTCTAGGGTGTAC
		GGCGGCAGCTGGTATGAGAGGCTCTGCGGC
		CCTTACACATACGAGTACAACTACTGGGGC
		CAAGGCACACAAGTGACTGTCTCGTCTGCT
		AGCCACCATCACCATCACCAC

377	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	279	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGCGGAGGAAGCGTG
		CAAGCCGGAGGATCTCTGAGACTGAGCTGC
		GCTGTGAGCGGCTACGCCTACTCCACATAC
		TGCATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAAGAGAGAGAGGGCGTGGCTGCTATCGAT
		AGCGGCGGCAGCACAAGCTACGCCGATAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGCCAAGAACACACTGTATCTGAGGATG
		AACTCTCTGAAGCCAGAGGACACAGCCATG
		TACTACTGTGCTGCTGTGCCTCCTCCTCCA
		GATGGCGGCAGCTGTCTGTTTCTGGGACCA
		GAGATCAAGGTCAGCAAGGCCGATTTTAGG
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

378	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	280	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTG
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		ACAGTGTCCGGCTACACTTACAGCTCCAAT
		TGCATGGGCTGGTTTAGGCAAGCCCCCGGC
		AAGGAAAGAGAGGGCGTGGCCACTATCTAC
		ACTGGCGGCGGCAACACATACTACGCCGAT
		AGCGTGAAGGGAAGGTTCACTATCAGCCAA
		GATAACGCCAAGAACACAGTGTATCTGCAG
		ATGAACAATCTGAAGCCAGAGGACACTGCC
		ATGTACTACTGTGCTGCTGAGCCACTGTCT
		AGGGTGTACGGCGGCAGCTGCCCAACTCCT
		ACATTCGACTACTGGGGCCAAGGCACACAA
		GTGACTGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

379	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	281	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTC
		CAAGCCGGAGGCTCTCTGAGGCTGAGCTGT
		GGAGCCAGCGGCTACACTTACAGCAGCTAC
		TGTATGGGCTGGTTTAGGCAAGTGCCCGGC
		AAGGAGAGAGAGGGCGTGGCCGTGATCGAT
		TCCGATGGCAGCACAAGCTACGCTGACAGC
		GTGAAGGGAAGGTTCACAATCAGCAAGGAC
		AACGGCAAGAACACACTCTATCTGCAGATG
		AACAGCCTCAAGCCAGAGGACACAGCCATG
		TACTACTGCGCCGCTGATCTGGGCCACTAT
		AGGCCTCCTTGTGGCGTGCTGTATCTGGGC
		ATGGATTACTGGGGCAAGGGCACACAAGTG
		ACAGTCTCGTCTGCTAGCCACCATCACCAT
		CACCAC

380	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGAGGA
	Sequence	AGCGTCCAAGCCGGAGGATCTCTGAGACTG
	Encoding	AGCTGCGCCGCTAGTGGCTACTCCTACAGC
	SEQ ID NO:	AGCTACTGCATGGGCTGGTTTAGGCAAGCC
	282	CCCGGCAAGGAGAGAGAAGGCGTGGCCACT
		ATCGACAGCGACGGCATGACAAGGTACGCC
		GACAGCGTGAAGGGAAGGTTCACAATCAGC
		AAGGACAACGCCAAGAACACACTGTATCTG
		CAGATGAACTCTCTGAAGCCAGAGGACACT
		GCCATGTACTACTGTGCCGCTCCTCTGTAC
		GACTGTGATAGCGGCGCTGTGGGCAGAAAT
		CCACCTTATTGGGGCCAAGGCACTCAAGTG
		ACAGTCTCGAGCGGCGGAGGATCCCAAGTG
		CAGCTGCAAGAGAGCGGAGGAGGAAGCGTC
		CAAGCCGGAGGCTCTCTGAGACTGAGCTGT
		GCCGCCAGCGGCTACTCCAACTGCAGCTAC
		GACATGACTTGGTATAGGCAAGCCCCCGGC
		AAGGAGAGGGAGTTCGTGTCCGCCATCCAC
		AGCGACGGCAGCACTAGATACGCCGACAGC
		GTGAAGGGAAGGTTCTTCATCAGCCAAGAT
		AACGCCAAGAACACAGTGTATCTGCAGATG
		AACTCCCTCAAGCCAGAGGACACTGCCATG
		TACTACTGCAAGACAGACCCACTGCACTGC
		AGAGCCCATGGCGGCAGCTGGTATAGCGTG
		AGGGCCAACTACTGGGGCCAAGGCACACAA
		GTGACAGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

381	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	283	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGAGGAGGAAGCGTGCAAGCC
		GGAGGCTCTCTGAGACTGAGCTGTGCCGCC
		TCTAGGTATCTGTACAGCATCGACTACATG
		GCTTGGTTCAGACAGAGCCCCGGCAAGGAG
		AGGGAGCCAGTGGCTGTCATCTACACTGCC
		TCCGGCGCCACATTCTATCCAGATAGCGTG
		AAGGGAAGGTTCACTATCAGCCAAGATAAC
		GCCAAGATGACAGTGTATCTGCAGATGAAC
		TCTCTGAAGAGCGAGGACACTGCCATGTAC
		TACTGTGCCGCCGTGAGGAAGACAGATAGC
		TACCTCTTCGACGCCCAGAGCTTCACATAC
		TGGGGCCAAGGCACACAAGTGACAGTCTCG
		TCTGCTAGCCACCATCACCATCACCAC

382	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	284	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGAGGAGGAAGCGTGCAAGCC
		GGAGGCTCTCTGAGGCTGAGCTGTGCCGCC
		TCTAGGTTCACATACAGCAGCTACTGCATG
		GGCTGGTTCAGACAAGCCCCCGGCAAAGAG
		AGAGAAGGCGTGGCCAGCATCGATAGCGAT
		GGCTCCACTAGCTACACTGACAGCGTGAAG
		GGAAGGTTCACTATCAGCAAGGACAACGCC
		AAGAACACTCTGTATCTGCAGATGAACTCT
		CTGAAGCCAGAGGACACAGCCATGTACTAC
		TGTGCCCTCGATCTGATGAGCACAGTGGTG
		CCCGGCTTCTGTGGCTTTCTGCTGAGCGCT
		GGCATGGATTACTGGGGCAAGGGCACTCAA
		GTGACTGTCTCGTCTGCTAGCCACCATCAC
		CATCACCAC

383	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	285	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGTCCGGAGGAGGCAGCGTCCAAGCC
		GGAGGCTCTCTGAGGCTGAGCTGTGCTGCC
		AGCGGCTACACTTACAGCATGTACTGCATG
		GGCTGGTTCAGACAAGCCCCCGGCAAGGAA
		AGAGAGGGCGTGGCCCAGATCAATAGCGAT
		GGCAGCACAAGCTACGCCGACAGCGTGAAG
		GGAAGGTTCACTATCTCCAAGGACAACGCC
		AAGAACACTCTGTATCTGCAGATGAACTCT
		CTGAAGCCAGAGGACACTGCCATGTACTAC
		TGCGCTGCCGATTCTAGGGTGTACGGCGGC
		AGCTGGTATGAGAGGCTCTGCGGCCCTTAC
		ACATACGAGTACAACTACTGGGGCCAAGGC
		ACACAAGTGACTGTCTCGTCTGCTAGCCAC
		CATCACCATCACCAC

384	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	286	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGCGGAGGAAGCGTGCAAGCC
		GGAGGATCTCTGAGACTGAGCTGCGCTGTG
		AGCGGCTACGCCTACTCCACATACTGCATG
		GGCTGGTTTAGGCAAGCCCCCGGCAAAGAG
		AGAGAGGGCGTGGCTGCTATCGATAGCGGC
		GGCAGCACAAGCTACGCCGATAGCGTGAAG
		GGAAGGTTCACAATCAGCAAGGACAACGCC
		AAGAACACACTGTATCTGAGGATGAACTCT
		CTGAAGCCAGAGGACACAGCCATGTACTAC
		TGTGCTGCTGTGCCTCCTCCTCCAGATGGC
		GGCAGCTGTCTGTTTCTGGGACCAGAGATC
		AAGGTCAGCAAGGCCGATTTTAGGTACTGG
		GGCCAAGGCACACAAGTGACAGTCTCGTCT
		GCTAGCCACCATCACCATCACCAC

385	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	287	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGAGGAGGAAGCGTGCAAGCC
		GGAGGCTCTCTGAGGCTGAGCTGTACAGTG
		TCCGGCTACACTTACAGCTCCAATTGCATG
		GGCTGGTTTAGGCAAGCCCCCGGCAAGGAA
		AGAGAGGGCGTGGCCACTATCTACACTGGC
		GGCGGCAACACATACTACGCCGATAGCGTG
		AAGGGAAGGTTCACTATCAGCCAAGATAAC
		GCCAAGAACACAGTGTATCTGCAGATGAAC
		AATCTGAAGCCAGAGGACACTGCCATGTAC
		TACTGTGCTGCTGAGCCACTGTCTAGGGTG
		TACGGCGGCAGCTGCCCAACTCCTACATTC
		GACTACTGGGGCCAAGGCACACAAGTGACT
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

386	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	288	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGAGGAGGAAGCGTCCAAGCC
		GGAGGCTCTCTGAGGCTGAGCTGTGGAGCC
		AGCGGCTACACTTACAGCAGCTACTGTATG
		GGCTGGTTTAGGCAAGTGCCCGGCAAGGAG
		AGAGAGGGCGTGGCCGTGATCGATTCCGAT
		GGCAGCACAAGCTACGCTGACAGCGTGAAG
		GGAAGGTTCACAATCAGCAAGGACAACGGC
		AAGAACACACTCTATCTGCAGATGAACAGC
		CTCAAGCCAGAGGACACAGCCATGTACTAC
		TGCGCCGCTGATCTGGGCCACTATAGGCCT
		CCTTGTGGCGTGCTGTATCTGGGCATGGAT
		TACTGGGGCAAGGGCACACAAGTGACAGTC
		TCGTCTGCTAGCCACCATCACCATCACCAC

387	DNA	CAAGTGCAGCTGCAAGAGAGCGGAGGCGGC
	Sequence	AGCGTGCAGACTGGAGGCTCTCTGAGACTG
	Encoding	AGCTGTGCTGCCAGCGGCTACACTTATCTG
	SEQ ID NO:	AGGGGCTGTATGGGCTGGTTTAGGCAAGCC
	289	CCCGGCAAGGAGAGAGAGGGCGTGGCCGTC
		ATGGATGTGGTGGGCGATAGGAGAAGCTAC
		ATCGACAGCGTGAAGGGAAGGTTCACAATC
		TCTAGGGACAATGCCGCCAACAGCGTCTAT
		CTGCAGATGGACAATCTGAAGCCAGAGGAC
		ACAGCCATGTACTACTGCACTGCCGGCCCT
		AACTGTGTGGGCTGGAGAAGCGGACTGGAT
		TACTGGGGCCAAGGCACACAAGTGACAGTC
		TCGAGCGGCGGAGGATCCCAAGTGCAGCTG
		CAAGAGAGCGGAGGAGGAAGCGTCCAAGCC
		GGAGGCTCTCTGAGACTGAGCTGTGCCGCC
		AGCGGCTACTCCAACTGCAGCTACGACATG
		ACTTGGTATAGGCAAGCCCCCGGCAAGGAG
		AGGGAGTTCGTGTCCGCCATCCACAGCGAC
		GGCAGCACTAGATACGCCGACAGCGTGAAG
		GGAAGGTTCTTCATCAGCCAAGATAACGCC
		AAGAACACAGTGTATCTGCAGATGAACTCC
		CTCAAGCCAGAGGACACTGCCATGTACTAC
		TGCAAGACAGACCCACTGCACTGCAGAGCC
		CATGGCGGCAGCTGGTATAGCGTGAGGGCC
		AACTACTGGGGCCAAGGCACACAAGTGACA
		GTCTCGTCTGCTAGCCACCATCACCATCAC
		CAC

388	SEQ ID NO:	IDYMA
	44 CDR 1

389	SEQ ID NO:	VIYTASGATFYPDSVKG
	44 CDR 2

390	SEQ ID NO:	VRKTDSYLFDAQSFTY
	44 CDR 3

391	SEQ ID NO:	SYCMG
	45 CDR 1

392	SEQ ID NO:	SIDSDGSTSYTDSVKG
	45 CDR 2

393	SEQ ID NO:	DLMSTVVPGFCGFLLSAGMDY
	45 CDR 3

394	SEQ ID NO:	MYCMG
	46 CDR 1

395	SEQ ID NO:	QINSDGSTSYADSVKG
	46 CDR 2

396	SEQ ID NO:	DSRVYGGSWYERLCGPYTYEYNY
	46 CDR 3

397	SEQ ID NO:	TYCMG
	47 CDR 1

398	SEQ ID NO:	AIDSGGSTSYADSVKG
	47 CDR 2

399	SEQ ID NO:	VPPPPDGGSCLFLGPEIK VSKADFRY
	47 CDR 3

400	SEQ ID NO:	SNCMG
	48 CDR 1

401	SEQ ID NO:	TIYTGGGNTYYADSVKG
	48 CDR 2

402	SEQ ID NO:	EPLSRVYGGSCPTPTFDY
	48 CDR 3

403	SEQ ID NO:	SYCMG
	49 CDR 1

404	SEQ ID NO:	VIDSDGSTSYADSVKG
	49 CDR 2

405	SEQ ID NO:	DLGHYRPPCGVLYLGMDY
	49 CDR 3

406	SEQ ID NO:	SYDMT
	50 CDR 1

407	SEQ ID NO:	AIHSDGSTRYADSVKG
	50 CDR 2

408	SEQ ID NO:	DPLHCRAHGGSWYSVRANY
	50 CDR 3

409	SEQ ID NO:	SGCMG
	51 CDR 1

410	SEQ ID NO:	AINSDGSTSYADSVKG
	51 CDR 2

411	SEQ ID NO:	EPYCSGGYPR
	51 CDR 3

412	SEQ ID NO:	SYCMG
	52 CDR 1

413	SEQ ID NO:	HIDSDGSTSYADSVKG
	52 CDR 2

414	SEQ ID NO:	DPIPGPGYCDGGPNKY
	52 CDR 3

415	SEQ ID NO:	SYCMG
	53 CDR 1

416	SEQ ID NO:	TIDSDGMTRYADSVKG
	53 CDR 2

417	SEQ ID NO:	DADCTIAAMTTNPL
	53 CDR 3

418	SEQ ID NO:	VNYMG
	54 CDR 1

419	SEQ ID NO:	TIFTGAGTTYYANSVKG
	54 CDR 2

420	SEQ ID NO:	DFRGGLLYRPAYEYTYR
	54 CDR 3

421	SEQ ID NO:	VNYMG
	55 CDR 1

422	SEQ ID NO:	TIFTGAGTTYYANSVKG
	55 CDR 2

423	SEQ ID NO:	DFRGGLLYRPAYEYTYR
	55 CDR 3

424	SEQ ID NO:	SYCMG
	56 CDR 1

425	SEQ ID NO:	TIDSDGMTRYADSVKG
	56 CDR 2

426	SEQ ID NO:	PLYDCDSGAVGRNPPY
	56 CDR 3

427	SEQ ID NO:	RGCMG
	57 CDR 1

428	SEQ ID NO:	VMDVVGDRRSYIDSVKG
	57 CDR 2

429	SEQ ID NO:	GPNCVGWRSGLDY
	57 CDR 3

430	ASH6	ASHHHHHH
	purification
	handle

It is understood that the embodiments described herein are for illustrative purposes only and that various modifications or changes in light thereof will be suggested to persons skilled in the art and are to be included within the spirit and purview of this application and scope of the appended claims. The sequences of the sequence accession numbers cited herein are hereby incorporated by reference.

Claims

What is claimed is:

1. An IL12 receptor (IL12R) binding protein that specifically binds to IL12Rβ1 and IL12Rβ2,

wherein the binding protein causes the multimerization of IL12Rβ1 and IL12Rβ2 and downstream signaling, and

wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL12Rβ1 (an anti-IL12Rβ1 sdAb) and a sdAb that specifically binds to IL12Rβ2 (an anti-IL12Rβ2 sdAb).

2. The IL12R binding protein of claim 1, wherein the anti-IL12Rβ1 sdAb is a V_HH antibody (an anti-IL12Rβ1 V_HH antibody) and/or the anti-IL12Rβ2 sdAb is a V_HH antibody (an anti-IL12Rβ2 V_HH antibody).

3. The IL12R binding protein of claim 1 or 2, wherein the anti-IL12Rβ1 sdAb and the anti-IL12Rβ2 sdAb are joined by a peptide linker.

4. The IL12R binding protein of claim 3, wherein the peptide linker comprises between 1 and 50 amino acids.

5. The IL12R binding protein of any one of claims 1 to 4, wherein the IL12R binding protein has a reduced E_maxcompared to IL12.

6. The IL12R binding protein of any one of claims 1 to 5, wherein the IL12R binding protein has a similar potency compared to that of IL12.

7. A method for treating cancer in a subject in need thereof, comprising administering to the subject the IL12R binding protein of any one of claims 1 to 6, wherein the IL12R binding protein binds to and activates natural killer, CD4⁺ T cells, and/or CD8⁺ T cells.

8. The method of claim 7, wherein the cancer is a solid tumor cancer.

9. An IL27 receptor (IL27R) binding protein that specifically binds to IL27Rα subunit (IL27Rα) and glycoprotein 130 subunit (gp130),

wherein the binding protein causes the multimerization of IL27Rα and gp130 and downstream signaling, and

wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL27Rα (an anti-IL27Rα sdAb) and a sdAb that specifically binds to gp130 (an anti-gp130 sdAb).

10. The IL27R binding protein of claim 9, wherein the anti-IL27Rα sdAb is a V_HH antibody (an anti-IL27Rα V_HH antibody) and/or the anti-gp130 sdAb is a V_HH antibody (an anti-gp130 V_HH antibody).

11. The IL27R binding protein of any one of claims 9 to 10, wherein the anti-IL27Rα sdAb and the anti-gp130 sdAb are joined by a peptide linker.

12. The IL27R binding protein of claim 11, wherein the peptide linker comprises between 1 and 50 amino acids.

13. A method for treating cancer in a subject in need thereof, comprising administering to the subject the IL27R binding protein of any one of claims 9 to 12, wherein the IL27R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, and/or T-regulatory (Treg) cells.

14. The method of claim 13, wherein the IL27R binding protein binds to and activates CD8⁺ T cells.

15. The method of claim 13 or 14, wherein the IL27R binding protein binds to and activates CXCR5⁺ CD8⁺ T cells.

16. The method of any one of claims 13 to 15, wherein the cancer is a solid tumor cancer.

17. An IL10 receptor (IL10R) binding protein that specifically binds to IL10Rα subunit (IL10Rα) and IL10Rβ,

wherein the binding protein causes the multimerization of IL10Rα and IL10Rβ and downstream signaling, and

wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL10Rα (an anti-IL10Rα sdAb) and a sdAb that specifically binds to IL10Rβ (an anti-IL10Rβ sdAb).

18. The IL10R binding protein of claim 17, wherein the anti-IL10Rα sdAb is a V_HH antibody (an anti-IL10Rα V_HH antibody) and/or the anti-IL10Rβ sdAb is a V_HH antibody (an anti-IL10Rβ V_HH antibody).

19. The IL10R binding protein of any one of claims 17 to 18, wherein the anti-IL10Rα sdAb and the anti-IL10Rβ sdAb are joined by a peptide linker.

20. The IL10R binding protein of claim 19, wherein the peptide linker comprises between 1 and 50 amino acids.

21. A method for treating cancer in a subject in need thereof, comprising administering to the subject the IL10R binding protein of any one of claims 17 to 20, wherein the IL10R binding protein binds to and activates CD8⁺ T cells, CD4⁺ T cells, macrophages, and/or Treg cells.

22. The method of claim 21, wherein the IL10R binding protein provides longer therapeutic efficacy than a pegylated IL10.

23. The method of claim 21 or 22, wherein the cancer is a solid tumor cancer.

24. An interferon (IFN) λ receptor (IFNλR) binding protein that specifically binds to IL10Rβ and IL28 receptor (IL28R) α subunit (IL28Rα),

wherein the binding protein causes the multimerization of IL10Rβ and IL28Rα and downstream signaling, and

wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to IL10Rβ (an anti-IL10Rβ sdAb) and a sdAb that specifically binds to IL28Rα (an anti-IL28Rα sdAb).

25. The IFNλR binding protein of claim 24, wherein the anti-IL10Rβ sdAb is a V_HH antibody (an anti-IL10Rβ V_HH antibody) and/or the anti-IL28Rα sdAb is a V_HH antibody (an anti-IL28Rα V_HH antibody).

26. The IFNλR binding protein of any one of claims 24 to 25, wherein the anti-IL10Rβ sdAb and the anti-IL28Rα sdAb are joined by a peptide linker.

27. The IFNλR binding protein of claim 26, wherein the peptide linker comprises between 1 and 50 amino acids.

28. A method for treating an infectious disease in a subject in need thereof, comprising administering to the subject an IFNλR binding protein of any one of claims 24 to 27, wherein the IFNλR binding protein binds to and activates macrophages, CD8⁺ T cells, CD4⁺ T cells, Treg cells, dendritic cells, and/or epithelial cells.

29. The method of claim 28, wherein the IFNλR binding protein binds to and activates macrophages.

30. The method of claim 28 or 29, wherein the infectious disease is influenza, hepatitis B, hepatitis C, or human immunodeficiency virus (HIV) infection.

31. A binding protein that specifically binds to IL10Rα and IL2Rγ,

wherein the binding protein causes the multimerization of IL10Rα and IL2Rγ and downstream signaling, and

wherein the binding protein comprises a sdAb that specifically binds to IL10Rα (an anti-IL10Rα sdAb) and a sdAb that specifically binds to IL2Rγ (an anti-IL2Rγ sdAb).

32. The binding protein of claim 31, wherein the anti-IL10Rα sdAb is a V_HH antibody (an anti-IL10Rα V_HH antibody) and/or the anti-IL2Rγ sdAb is a V_HH antibody (an anti-IL2Rγ V_HH antibody).

33. The binding protein of any one of claims 31 to 32, wherein the anti-IL10Rα sdAb and the anti-IL2Rγ sdAb are joined by a peptide linker.

34. The binding protein of claim 33, wherein the peptide linker comprises between 1 and 50 amino acids.

35. A method for treating cancer in a subject in need thereof, comprising administering to the subject the binding protein of any one of claims 31 to 34, wherein the binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells.

36. The method of claim 35, wherein the method does not cause anemia.

37. A binding protein that specifically binds to a first receptor and a second receptor,

wherein the first receptor is interferon γ receptor 1 (IFNγR1) or IL28Rα and the second receptor is preferentially expressed on myeloid cells and/or T cells,

wherein the binding protein causes the multimerization of the first receptor and the second receptor and their downstream signaling, and

wherein the binding protein comprises a single-domain antibody (sdAb) that specifically binds to the first receptor and a sdAb that specifically binds to the second receptor.

38. The binding protein of claim 37, wherein the sdAb that specifically binds to the first receptor is an anti-IFNγR1 V_HH antibody.

39. The binding protein of claim 37, wherein the sdAb that specifically binds to the first receptor is an anti-IL28Rα V_HH antibody.

40. The binding protein of any one of claims 37 to 39, wherein the first receptor is IFNγR1 and the second receptor is IL2Rγ.

41. The binding protein of any one of claims 37 to 39, wherein the first receptor is IL28Rα and the second receptor is IL2Rγ.

42. The binding protein of any one of claims 37 to 41, wherein the sdAb that specifically binds to the first receptor and the sdAb that specifically binds to the second receptor are joined by a peptide linker.

43. The binding protein of claim 42, wherein the peptide linker comprises between 5 and 50 amino acids.

44. A method for treating cancer in a subject in need thereof, comprising administering to the subject the binding protein of any one of claims 37 to 43, wherein the binding protein binds to and activates myeloid cells and/or T cells.

45. The method of claim 44, wherein the binding protein binds to and activates macrophages.

46. The method of claim 44, wherein the binding protein binds to and activates CD8⁺ T cells and/or CD4⁺ T cells.

47. The IL10R binding protein of any one of claims 17 to 20 wherein the anti-IL10Rα sdAb is selected from the group consisting of SEQ ID NOs: 44-50 and the anti-IL10Rβ sdAb is selected from the group consisting of SEQ ID Nos: 51-57.

48. The IL10R binding protein of claim 47 wherein the anti-IL10Rα sdAb is joined to the anti-IL10Rβ sdAb via a linker selected from the group consisting of SEQ ID Nos: 1-23.

49. The ILR binding protein of claim 47 wherein the IL10R binding protein comprises, from amino to carboxy, a first anti-IL10R sdAb joined via a linker to a second anti-IL10R sdAb, according to the following:


	first anti-IL10R	second anti-IL10R
	sdAb SEQ ID	sdAb SEQ ID

	48	57
	49	56
	50	55
	52	46
	47	51
	51	47
	46	55
	46	56
	47	56
	46	54
	44	53
	55	44
	46	52
	45	57
	45	55
	47	55
	50	54
	48	55
	46	57
	47	57
	50	56
	49	51
	52	45
	53	44
	54	47

and wherein said linker is selected from the group consisting of SEQ ID Nos:1-23.

50. The IL-10 receptor binding protein of claim 17 selected from the group consisting of SEQ ID Nos: 194, 209, 210, 211, 213, 218, 226, 233, 238, 244, 250, 203, 205, 207, 269, 212, 217, 219, 224, 227, 237, 239, and 249.

Resources

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COMPOSITIONS AND METHODS RELATED TO RECEPTOR PAIRING

COMPOSITIONS AND METHODS RELATED TO RECEPTOR PAIRINGS

Abstract:

Inventors:

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Description

CROSS-REFERENCE TO RELATED PATENT APPLICATIONS

SEQUENCE LISTING

BACKGROUND OF THE DISCLOSURE

SUMMARY OF THE DISCLOSURE

DETAILED DESCRIPTION OF THE DISCLOSURE

I. Introduction

II. Definitions

III. Compositions and Methods

IL12 Receptor Binding Proteins

IL27 Receptor Binding Proteins

IL10 Receptor Binding Proteins

IFNλ Receptor Binding Proteins

IL23 Receptor Binding Proteins

IL2 Receptor Binding Proteins

IL22 Receptor Binding Proteins

IV. Single-Domain Antibody and VHH

V. Linkers

VI. Modifications to Extend Duration of Action In Vivo

VII. Pharmaceutical Composition

VIII. Indications

EXAMPLES

Example 1—VhH Generation

Example 2. Generation of Anti-hIL10R VHHs

Example 3. Synthesis of DNA Encoding Synthekines

Example 4. Recombinant Production and Purification

Example 5. IL10 Activity Assay

Example 6. Screening of SEQ ID NOs: 192-289

Claims

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IV. Single-Domain Antibody and V_HH

Example 1—V_hH Generation